Abstract
Following CART-19 immunotherapy for B-cell acute lymphoblastic leukaemia (B-ALL), many patients relapse due to loss of the cognate CD19 epitope. Since epitope loss can be caused by aberrant CD19 exon 2 processing, we herein investigate the regulatory code that controls CD19 splicing. We combine high-throughput mutagenesis with mathematical modelling to quantitatively disentangle the effects of all mutations in the region comprising CD19 exons 1-3. Thereupon, we identify ~200 single point mutations that alter CD19 splicing and thus could predispose B-ALL patients to developing CART-19 resistance. Furthermore, we report almost 100 previously unknown splice isoforms that emerge from cryptic splice sites and likely encode non-functional CD19 proteins. We further identify cis-regulatory elements and trans-acting RNA-binding proteins that control CD19 splicing (e.g., PTBP1 and SF3B4) and validate that loss of these factors leads to pervasive CD19 mis-splicing. Our dataset represents a comprehensive resource for identifying predictive biomarkers for CART-19 therapy.
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Introduction
B-cell acute lymphoblastic leukemia (B-ALL) is a haematologic malignancy that causes a significant number of childhood and adult cancer deaths. During CART-19 immunotherapy, chimeric antigen receptor-armed autologous T-cells (CARTs) are engineered to target the surface antigen CD19 on B cells by linking the single-chain variable fragment (scFv) of an anti-CD19 antibody to the intracellular signalling domain of the T-cell receptor1. Upon CD19 recognition, the chimeric antigen receptors activate the cytotoxic T-cells to attack the tumour cells. CART-19 therapy was recently approved for the treatment of paediatric B-ALL in the US and Europe, achieving initial remission rates up to 90%2. This indicates that B-ALL cells at initial screening are typically CD19-positive. Unfortunately, up to 50% of children relapse under CART-19 therapy, and response rates are even worse in adults3,4. Several studies reported that in 40–60% of relapse cases, the cancerous B cells become invisible to the CARTs because they lose expression of the CD19 epitope (CD19-negative)5,6,7,8. This recurrently involves alternative splicing of the CD19 pre-mRNA9,10,11.
Splicing involves the excision of introns and the joining of exons by the spliceosome to generate mature mRNAs. In alternative splicing, certain exons can be either included or excluded (“skipped”), resulting in different transcript isoforms. The splicing outcome at each exon is controlled by a large set of cis-regulatory elements in the RNA sequence which are recognised by trans-acting RNA-binding proteins (RBPs) that guide the spliceosome activity. It is increasingly recognised that widespread alterations in splicing are a molecular hallmark of cancer and often contribute to therapeutic resistance (reviewed in ref. 12). For instance, intron retention, i.e., the failure to remove certain introns, often disrupts the open reading frame (ORF) with premature termination codons (PTCs) and thereby compromises the expression of the encoded proteins. Consistent with the widespread splicing changes, cancer-causing driver mutations frequently occur in splice-regulatory cis-elements, and many splicing factors have oncogenic properties, being commonly mutated or dysregulated in cancer12,13,14.
Multiple alternative splicing events in CD19 mRNA have been described to interfere with CART-19 therapy9,11,15,16,17,18. Most prominently, skipping of exon 2 results in a truncated CD19 protein which is no longer presented on the cell surface and hence fails to trigger CART-19-mediated killing9,15. In addition, it was reported that relapsed patients showed retention of intron 2 which introduces a PTC, thereby disrupting CD19 expression11. Similarly, simultaneous skipping of exons 5 and 6 introduces a PTC9. The splicing alterations can be caused by mutations within the CD19 gene or by changes in the expression of trans-acting RBPs. For instance, it has been shown that the known splicing regulator SRSF3 binds to cis-regulatory elements within CD19 exon 2 to promote its inclusion9. Of note, alternative CD19 isoforms showing exon 2 skipping were observed to pre-exist in patients prior to CART-19 therapy16, suggesting that CD19 splicing patterns may harbour predictive information and could be modulated to re-establish sensitivity to CART-19-mediated killing. However, Orlando and co-workers suggested that alternative splicing changes in B-ALL patients are present in diagnostic samples already (albeit at low frequencies) and may not contribute meaningfully to CD19 epitope loss5. We, therefore, set out to investigate CD19 alternative splicing and its molecular determinants in B-ALL in more detail.
High-throughput mutagenesis screens combined with next-generation sequencing provide comprehensive insights into the regulatory code of splicing19,20,21,22. The interpretation of such data is challenging, as the mutation effects often depend on other mutations and are typically most pronounced at intermediate exon inclusion levels19,20,23. We and others have shown by mathematical modelling that kinetic models account for the context-dependence of mutation effects on splice isoforms19,20. By utilising these models, systems-level insights can be gained into complex cis-regulatory landscapes, effects of trans-acting RBPs, and principles of splicing regulation19,20,24.
In this work, we combine B-ALL patient data with high-throughput mutagenesis, mathematical modelling and RBP knockdowns to comprehensively characterise cis-regulatory mutations and trans-acting RBPs controlling CD19 exon 2 splicing. Unlike previous mutagenesis screens, we determine all intronic and exonic mutation effects in a 1.2 kb region and quantify the abundance of 100 alternative isoforms, including intron 2 retention and alternative 3′/5′ splice site usage. Many of these isoforms encode for a non-functional CD19 protein and are therefore likely to impair CART-19 therapy. By in silico analyses and RBP knockdowns, we identify trans-regulators of CD19 splicing that promote the production of the therapy-impacting isoforms. Taken together, our dataset allows for a systems-level understanding of the splicing code and provides a comprehensive resource of predictive markers for CART-19 therapy resistance.
Results
CART-19 patients show increased CD19 intron 2 retention after relapse
To resolve the contribution of CD19 splicing in CART-19 therapy, we re-analysed RNA-seq data from Orlando and co-workers5, in which B-ALL cells of 17 patients were sequenced at initial screening and after relapse. In contrast to the original study, we expanded the analyses to intron retention events surrounding CD19 exon 2. We found that the average frequency of intron 2 retention across patients is unexpectedly high (63%) before therapy and significantly increases to 82% after relapse (P value = 0.009, Wilcoxon signed-rank test; Fig. 1a, b). The trend towards higher intron 2 retention in the therapy-resistant tumours is preserved in seven out of nine individual patients that were sequenced both before therapy and after relapse (Fig. 1b). Since the resulting isoform does not encode a functional CD19 protein, this suggests that increased intron 2 retention contributes to CART-19 therapy resistance, as reported in a recent study11.
Given the high prevalence of intron 2 retention even before CART-19 therapy, we extended our analysis to 220 B-ALL patients from the Therapeutically Applicable Research To Generate Effective Treatments (TARGET) programme. Although these patients had not been treated with CART-19, intron 2 retention appears as the predominant isoform in almost all of them (Fig. 1c, Supplementary Fig. 1a, b). This suggests that the cancer cells generally exhibit CD19 mis-splicing. Interestingly, strong intron 2 retention is also observed in immature B-cell precursors from healthy donors, whereas it is negligible in mature B cells (Fig. 1d). Therefore, incomplete B-cell differentiation in B-ALL may be accompanied by CD19 mis-splicing which is further aggravated during CART-19 therapy.
Somatic mutations in relapsed patients cause splicing alterations
To learn about the genetic causes of the splicing alterations during relapse, we took a closer look at the mutations accumulating in the B-ALL patients of the Orlando study5. The majority of relapsed patients (12 out of 17) harbour somatic mutations within the CD19 gene, including frameshift insertions, deletions and single nucleotide missense variants. We selected nine mutations in exons 2 or 3 from eight patients for further analysis (Supplementary Table 1). To test for effects on splicing, we constructed a minigene reporter that harbours CD19 exon 1–3 including the two intervening introns 1 and 2 (Fig. 1e). We confirmed that the minigene gives rise to the same transcript isoforms with quantitatively similar frequencies as the endogenous gene in the human B-ALL cell line NALM-6 (Fig. 1f, g, Supplementary Fig. 1c).
When introducing the patient mutations into our minigene reporter, we found that six out of nine tested mutations lead to the production of alternative CD19 isoforms linked to CART-19 therapy resistance (Fig. 1h, i, Supplementary Fig. 1d): The mutation from patient #2 induces exon 2 skipping, while mutations from patients #4 and #14 (#14.2) cause intron 2 retention. The latter mirrors the increase of this isoform in the same patients after CART-19 therapy relapse (Fig. 1b). In addition, three mutations enhance the production of an additional isoform that uses an alternative 3′ splice site in exon 2 (termed alt-exon2; mutations from patients #5, #14.1 and #15). We note that as reported by Orlando and co-workers5, most of the patient mutations also introduce frameshifts and therefore perturb CD19 protein expression by disrupting the open reading frame. Interestingly, splicing effects and frameshifts potentially interact in a non-intuitive way: For instance, the deletion in patient #5 causes a frameshift, but at the same time activates an alternative 3′ splice site (alt-exon2) which restores the open reading frame (Supplementary Fig. 1e). Thus, taking splicing information into account is essential to understand whether a targetable CD19 protein is generated in a patient harbouring CD19 mutations.
High-throughput screening of alternative splicing of CD19 exons 1–3
To systematically study the effects of point mutations on CD19 exons 1–3 splicing, we adopted our previously developed massively parallel splicing reporter assay19 (Fig. 2a). To this end, we randomly introduced point mutations as well as short insertions and deletions into the CD19 minigene reporter by error-prone PCR. This yielded a pool of 10,295 minigene variants, each with a different set of mutations and tagged with a unique 15-nt barcode sequence. As an internal control, 194 wild type (WT) minigenes with distinct barcodes were added. Mutations in all minigene variants were mapped using targeted long-read DNA sequencing (DNA-seq, PacBio SMRT-seq, Supplementary Fig. 2a, b) and validated for 30 minigene clones via Sanger sequencing. The DNA-seq data shows that the minigene variants contain on average 9.7 mutations (Supplementary Fig. 2c). This allows for a comprehensive characterisation of the mutation landscape, as each position is on average mutated in 80 different minigene variants and 90% of the mutations are present in at least four distinct minigene variants (Supplementary Fig. 2d, e). To measure splicing outcomes, the minigene pool was transfected into NALM-6 cells and the resulting transcripts were quantified by targeted RNA sequencing (RNA-seq) using 350 nt + 250 nt paired-end reads (Illumina MiSeq, Supplementary Figs. 2a, 3a). We detected around 100 different splice isoforms (see below) which were unambiguously identified by paired-end sequencing. Two replicate experiments showed a high correlation in the measured isoform frequencies (R between 0.91 and 0.98 for the different isoforms, Supplementary Fig. 3b). Based on the common barcode sequence, information from DNA and RNA sequencing could be combined, linking mutations at the DNA level to frequencies of RNA splice isoforms for a total of 10,295 minigenes in two replicate experiments (Supplementary Data 1).
Therapy-impacting isoforms accumulate in response to numerous point mutations
To our surprise, the screen revealed a high complexity of CD19 exon 1–3 splicing, with a total of 101 alternative isoforms occurring with a frequency of ≥5% of all transcripts in at least two minigene variants (Supplementary Data 2). Out of these, the five major isoforms exceed 1% in WT minigenes, whereas the others, termed cryptic isoforms, only accumulate in mutated minigene variants (Fig. 2b). In WT, the most abundant major isoform by far is exon 2 inclusion (termed “inclusion”), followed by exon 2 skipping (termed “skipping”) and intron 2 retention (termed “intron2-retention”). Two additional major isoforms in WT originate from alternative 3′ splice site usage within exon 2 (alt-exon2) and 3 (alt-exon3) (Fig. 2b, c). Notably, alt-exon2 uses the same splice junction that we had observed upon introducing patient mutations into the CD19 minigene (Fig. 1i). As expected, the measured frequencies for the major isoforms show little variance for the 194 unmutated WT minigenes (standard deviation <6%, Fig. 2c). In contrast, many mutated minigene variants show strong changes relative to WT, suggesting a large impact of specific mutations on splicing outcomes (Fig. 2c). For instance, all minigenes with a mutation in the 3′ splice site of exon 2 lose the inclusion isoform, accompanied by strong alterations in the remaining major isoforms. Taken together, these observations support the accuracy of our screening results.
All major isoforms, except exon 2 inclusion, could contribute to therapy resistance either by generating an altered CD19 protein lacking a functional CART-19 epitope or by decreasing its production. Our unbiased screening approach extends the list of potentially therapy-impacting CD19 mutations, since 1721 out of 9127 mutated minigenes show exon 2 skipping, intron 2 retention and/or alt-exon2 isoform frequencies of >25% (Fig. 2c). However, since the minigene variants carry on average 9.7 point mutations, the observed splicing changes represent the combined effects of several mutations. To extract the impact of individual mutations, we adapted our previous mathematical modelling framework19 and implemented a multinomial logistic regression approach. Here, the splicing change in each minigene variant is described as the sum of the underlying point mutation effects (Fig. 3a, see Methods). These single-mutation effects are unknown and are determined by simultaneously fitting the model to all minigene measurements. Thereby, we were able to infer the individual effects of 4255 point mutations on the five major isoforms (Fig. 3a, Supplementary Fig. 4a). We validated the reliability of this model in describing combined mutations using a 10-fold cross-validation approach, in which we left out 10% of all minigene variants from fitting and were able to accurately predict them after model fitting (Pearson correlation coefficients 0.68–0.95; Fig. 3b, Supplementary Fig. 4b). In particular, isoforms abundant in WT or strongly accumulating in response to a large number of mutations (inclusion, skipping and alt-exon3) were predicted with high accuracy, whereas the prediction power was slightly lower for isoforms with a worse signal-to-noise ratio (intron2-retention and alt-exon2; Fig. 2c). Furthermore, we estimated that the model performed well in predicting single-mutation effects, as soon as a mutation occurred in three or more minigenes in the dataset (Supplementary Fig. 4c), which applied to 90% of all mutations (Supplementary Fig. 2e).
Out of 4255 quantified single-mutation effects, we find 193 splicing-affecting mutations that significantly alter the frequency of at least one isoform in the two replicates beyond the 2.5 and 97.5% quantiles of the WT minigene distribution (Fig. 3c, Supplementary Data 3, Source Data file). 37 of these splicing-affecting mutations overlap with single nucleotide variants (SNVs) that were previously reported in the human population from whole-genome or exome sequencing data, as well as reported cancer-associated mutations, with some of them predicted to have a pathogenic or likely pathogenic effect in the disease context (Supplementary Data 3). The strongest mutation effects accumulate around the four main splice sites and throughout exon 2 and correspond to the core cis-regulatory elements, such as splice site dinucleotides, branchpoint and polypyrimidine tract, as well as auxiliary elements (Fig. 3c, d). In particular, 21% of all positions within exon 2 (55 out of 267 nt) harbour at least one splicing-affecting mutation for any isoform, suggesting that CD19 exon 2 is densely packed with cis-regulatory elements.
Inspecting in more detail the 83 mutations that specifically impact CD19 exon 2 skipping, we find them to cluster within and around exon 2 (odds ratio 2.06 for such mutations to occur inside exon 2, P value = 0.002614, Fisher’s exact test). In addition, we observe smaller clusters of mutations within the introns and flanking constitutive exons which likely represent more distal cis-regulatory elements (Fig. 3c). Similarly, we explored the 54 splicing-affecting mutations impacting on intron2-retention. As expected, strongest effects are observed at the splice sites of intron 2. In addition, we find clusters of splicing-affecting mutations in intron 2 and exon 3 that might reflect important cis-regulatory elements. The predicted effects of all mutations on the five major isoforms can be explored in the associated Source Data file.
To test a subset of the regression predictions, we generated 19 minigenes with individual point mutations that are predicted to affect at least one isoform, including two previously reported SNVs (Supplementary Fig. 5a, Supplementary Data 4). Using semiquantitative RT-PCR, we were able to confirm that mutations near the splice sites of exon 2 predominantly lead to exon 2 skipping, whereas mutations in exon 3 result in intron2-retention and/or alt-exon3 formation (Fig. 3e, Supplementary Fig. 5b). Overall, the splicing measurements for the individual minigenes show high correlation with the regression predictions for the respective mutations across all five major isoforms (Fig. 3f, Supplementary Fig. 5c). In conclusion, our combined screening and modelling approach quantitatively describes alternative splicing of CD19 exons 1–3 by predicting the effects of all individual point mutations and combinations thereof. Our screen thereby represents a comprehensive resource for the identification of mutations with potential clinical relevance in CART-19 therapy resistance.
Cryptic isoforms destroy the CD19 ORF and are associated with recurrent mutations
Besides the five major isoforms, the CD19 exons 1–3 can give rise to 96 cryptic isoforms which are rare (<1%) in WT, but accumulate upon certain mutations (Fig. 2b, Supplementary Data 2). The cryptic isoforms involve a total of 71 cryptic splice sites (Fig. 4a). Of note, 33 of these cryptic isoforms make up >50% of total transcripts and are therefore dominant in certain minigene variants (Fig. 2b, c). To assess whether these cryptic isoforms impact on CD19 epitope presentation, we analysed their coding potential and found that the vast majority of cryptic CD19 isoforms (78 out of 96) show a frameshift and/or carry a PTC (Fig. 4b). This will either lead to the production of truncated CD19 peptides that likely do not allow for presentation on the cell surface15 or will induce nonsense-mediated mRNA decay of the cryptic isoforms and will hence reduce CD19 transcript and protein levels.
To derive a mechanistic understanding of cryptic isoform biogenesis, we analysed the underlying point mutations. To this end, we calculated a prevalence score which quantifies the degree of association between an isoform and a point mutation by multiplying: (i) the frequency of a mutation being present if the isoform level is high (>5%), and (ii) the frequency of the isoform level being high given that the mutation is present. A prevalence score of 1 indicates perfect correspondence between mutation and isoform, whereas a prevalence score of 0 is observed if they are unrelated. This score-based analysis revealed 38 mutation-isoform pairs with prevalence scores > 0.25 which could explain the genesis of 36 cryptic isoforms based on 31 point mutations (Supplementary Fig. 6a, Supplementary Data 2). The remaining 60 cryptic isoforms do not show a specific association, implying that they can either be generated by multiple redundant mutations, or that our screen lacks sufficient coverage to support a reliable association. To directly test the predicted associations, we introduced five mutations with a specific association to a cryptic isoform in our minigene reporter (C535G, chr16:28932405, prevalence score = 0.18; C806A, chr16:28932676, 0.68; A827T, chr16:28932697, 0.93; C864G, chr16:28932875, 1; G1005A, chr16:28932734, 0.89). Semiquantitative RT-PCR confirmed that all five tested mutations lead to the appearance of the associated cryptic isoform (Fig. 4c, d).
Altogether, our analysis provides a list of 31 mutations that are likely to trigger cryptic isoform formation. Importantly, the resulting cryptic isoforms show a maximum usage of up to 91% (Supplementary Data 2), which is expected to drastically interfere with normal CD19 splicing, protein production, and subsequent epitope presentation. Screening for the occurrence of the 96 cryptic isoforms in the TARGET B-ALL patient samples, we readily detected two junctions of cryptic isoforms that had been present already prior to CART-19 therapy (Fig. 1c, Supplementary Fig. 1a). Other cryptic isoforms predicted from our screen were not found in these patients that had not been treated with CART-19 therapy, but could already exist subclonally and/or may only emerge under the selective pressures of CD19-directed immunotherapy. The same applies to the associated mutations identified from our screen which were also not present in the TARGET B-ALL data (Supplementary Data 4).
The cryptic isoforms are caused by mutations that disrupt or create splice sites
Due to their potential clinical relevance, we wanted to learn more about how the mutations activate the cryptic isoforms. We found that the majority of mutations with a prevalence score > 0.25 are either in close proximity or directly overlap with the associated cryptic splice site (77.4% with distance <5 nt; odds ratio 7.55, P value = 1.793e-07, Fisher’s exact test; Fig. 4e). Further inspection showed that the underlying mutations either destroy the original splice site (7.9%) or generate a new cryptic splice site (57.9%). Hence, the cryptic isoforms do originate from the generation or destruction of core cis-regulatory elements rather than affecting auxiliary elements.
Currently, major efforts are ongoing to implement artificial intelligence (AI) tools to predict the effect of clinical variants on the splicing outcome. We therefore tested whether the state-of-the-art neural network SpliceAI25, which predicts changes in the splicing patterns induced by single point mutations, captures the gain and loss of splice sites in CD19. We applied SpliceAI using all possible single-point mutations in the CD19 minigene as an input. Similar to the results from our mutagenesis screen (Fig. 4a), SpliceAI predicts cryptic splice site activation by mutations throughout the minigene, with an increased density around the 3′ splice site of exon 3 (Supplementary Fig. 6b). All SpliceAI-predicted mutations are close to the affected cryptic splice sites (Supplementary Fig. 6c). Hence, SpliceAI successfully reflects the global landscape of mutation-induced cryptic splice site activation in the CD19 minigene.
With respect to the accuracy of the individual predictions, we found that 10 out of 38 mutations with strong SpliceAI predictions (SpliceAI score > 0.5) indeed lead to the accumulation of splice isoforms with the corresponding cryptic splice sites in the experimental data (prevalence score > 0.25, Fig. 4f). In the remaining 28 cases, either weak overall cryptic splice site activation occurred in the data (9 cases) or a different cryptic splice site was activated than predicted by SpliceAI (19 cases; Supplementary Fig. 6b). In quantitative terms, the likelihood of a cryptic splice site activation according to the SpliceAI prediction (“SpliceAI score”) is correlated to the magnitude of the prevalence score linking the mutation to the corresponding cryptic isoform in our screen (Fig. 4f). Overall, the comparison supports that SpliceAI can guide the interpretation of mutation effects in clinical samples, though direct experimental validation is necessary. Due to the robust performance of SpliceAI, we decided to predict splice-changing mutations throughout the entire CD19 gene and overlapped them with publicly reported single nucleotide variants (SNVs; Supplementary Fig. 6c). These predictions and variant overlap are provided as a resource (Supplementary Data 5) and can be used to evaluate the impact of new patient mutations on CD19 splicing in the future.
From our mutagenesis data, we found that the cryptic isoforms arise from numerous 3′ and 5′ cryptic splice sites that distribute over the entire minigene and accumulate at exon 3 (Fig. 4a). In line with their high prevalence, 26 cryptic splice sites reach >50% usage upon certain mutations, particularly around the start of exon 3. We hypothesised that cryptic splice site activation occurs in exon 3 because its canonical splice site can be outcompeted by neighbouring cryptic sites. To test this, we scored the strength of local consensus sequences using MaxEntScan26, and indeed found that the 3′ splice site of exon 3 is weak compared to all other canonical splice sites of CD19 exons 1–3 (Fig. 4g, Supplementary Fig. 6e, f). In line with our hypothesis, mutations around the 3′ splice site of exon 3 frequently create stronger splice sites than elsewhere in the minigene that exceed the strength of the canonical 3′ splice site of exon 3 (Fig. 4g). This suggests that weak splice sites are particularly vulnerable to the activation of competing cryptic splice sites and should be of particular interest when assessing the impact of clinical variants on splicing outcomes.
An extensive network of RBP regulators might drive CD19 mis-splicing
Besides CD19 mutations, CART-19 therapy resistance may also stem from altered expression of trans-acting RBPs which bind to the CD19 pre-mRNA to control alternative splicing. To identify putative RBP regulators, we explored publicly available databases containing experimentally determined RBP binding motifs (ATtRACT27 and oRNAment28). Furthermore, we included RBP binding information from the public resource of ENCODE eCLIP datasets29. Since the CD19 mRNA is hardly expressed in the ENCODE cell lines and binding events in CD19 can therefore not be directly extracted, we employed the prediction algorithm DeepRiPe30. The underlying neural network has been trained on the PAR-CLIP and ENCODE eCLIP datasets and thereby allows to predict changes of RBP binding upon mutation in any RNA sequence. In combination, these tools predict a total of 198 RBPs to bind within CD19 exons 1–3 (ATtRACT: 62 RBPs; oRNAment: 70 RBPs) or to decrease (or increase) binding upon mutation (DeepRiPe: 128 RBPs; Fig. 5a, b, Supplementary Fig. 7a).
To link the putative RBP regulators to the observed splicing changes, we overlaid the predicted binding sites (or predicted mutations for DeepRiPe) with splicing-affecting mutations from our screen. Overall, we find that 79% and 60% of ATtRACT and oRNAment binding sites, respectively, overlap with a splicing-affecting mutation (affecting any of the five major isoforms). Furthermore, 105 (5%) of the mutations predicted to change RBP binding by DeepRiPe overlap with splicing-affecting mutations, suggesting that modulating RBP binding at these sites may have a functional impact on CD19 splicing (Fig. 5c, Supplementary Fig. 7a). By merging these sets, we obtained a list of 119 RBPs that may regulate splicing by binding to CD19 exons 1–3 (Supplementary Data 6). Most of these are expressed in cancerous B cells from B-ALL patients from31 (80 with mean FPKM [fragments per kilobase of transcript per million mapped reads] > 10; Supplementary Fig. 7b) and could thus modulate CD19 splicing. Among these RBPs are SRSF3, a previously reported regulator of CD19 splicing9, but also new candidates such as PTBP1. Overall, the in silico predictions suggest the presence of an extensive RBP network that controls CD19 splicing and may impact the CART-19 therapy success.
Depletion of PTBP1 and several other RBPs results in non-functional CD19 isoforms
Based on our experimental data, in silico predictions, expression, literature information and manual curation, we shortlisted 11 RBP candidates for further analysis, including SRSF3 as a positive control (Fig. 5d). All 11 RBPs are expressed in normal B cells and B-ALL patient samples from the TARGET B-ALL cohort (Supplementary Fig. 8a). To test their impact on endogenous CD19 splicing, we generated NALM-6 cell lines stably expressing shRNAs against the shortlisted RBPs (depletion to <40% transcripts; Supplementary Fig. 8b). As previously described9, knockdown of SRSF3 leads to increased exon 2 skipping in the endogenous CD19 transcripts, confirming that this SR protein is required for exon 2 inclusion (Fig. 5e, f). Importantly, we find that knockdown of six additional RBPs (PTBP1, PCBP2, SF3B4, HNRNPK, MBNL1 and HNRNPM) has significant effects on CD19 alternative splicing (Fig. 5e, f, Supplementary Fig. 8c, d). The knockdown of these factors reduces CD19 exon 2 inclusion, while promoting intron2-retention and/or exon 2 skipping, thus shifting the cells towards expression of the relapse-associated CD19 isoforms. This implies that reduced levels of these factors can impair targetable CD19 epitope expression.
PTBP1 stands out among the putative regulators as it shows the strongest effects on intron2-retention. This splicing event introduces a premature termination codon that likely reduces CD19 transcript and protein expression via nonsense-mediated mRNA decay (Fig. 2b). In line with a role of PTBP1 in CD19 mis-splicing in tumours, we find that patient samples from the TARGET B-ALL cohort on average show lower PTBP1 mRNA expression compared to healthy B cells (Supplementary Fig. 8a). Within the B-ALL samples, PTBP1 expression negatively correlates with CD19 intron2-retention, as expected based on our knockdown experiments (R = -0.24; Fig. 6a, left). In addition, we investigated PTBP2 mRNA expression, which is tightly repressed by the PTBP1 protein via alternative splicing and nonsense-mediated mRNA decay32 and hence serves as a direct sensor for PTBP1 activity in the cells. Indeed, we find a strong correlation between increased PTBP2 mRNA levels, i.e., lowered PTBP1 protein activity, and increased CD19 intron2-retention (R = 0.56; Fig. 6a, right). To test for changes upon CART-19 relapse, we extracted PTBP1 and PTBP2 from expression data provided by the Orlando study5. Although we do not detect systematic changes in the PTBP1 mRNAs levels, the PTBP2 mRNA levels are significantly increased at relapse relative to screening, possibly indicating lowered PTBP1 protein levels (P value = 0.037, Wilcoxon rank-sum test; Fig. 6b). Together, these analyses suggest that PTBP1 is a regulator of CD19 alternative splicing, which we decided to explore further.
PTBP1 recognises clusters of UC-rich motifs33,34. Remarkably, ATtRACT predicts almost 100 such PTBP1 binding motifs across the studied CD19 region, including 25 that overlap with splicing-affecting mutations (Fig. 5d, Supplementary Data 6). Moreover, DeepRiPe predicts 78 mutations in 63 positions that change PTBP1 binding, out of which 10 are splicing-affecting in our screen (odds ratio 3.21, P value = 0.002481, Fisher’s exact test). The high number of predicted binding sites suggests a partial redundancy, indicating that PTBP1 regulation might be difficult to disrupt with individual point mutations as introduced in our screen. To experimentally test if PTBP1 binds to the predicted sites, we performed PTBP1 iCLIP2 experiments35 in NALM-6 cells. In line with a role in intron2-retention, we find extensive PTBP1 binding, particularly in intron 2, where it spreads over an extended cluster of predicted binding sites (Fig. 6c). This suggests that PTBP1 directly regulates CD19 splicing via intron 2 binding.
Next, we chose to assess whether PTBP1-mediated splicing changes affect CD19 surface exposure on B cells. To test this, we performed siRNA-mediated knockdown of PTBP1 in P493-6 and MHHCALL4 cells (Supplementary Fig. 9a, b) and confirmed that the knockdown increased levels of CD19 intron2-retention in both cell lines (Supplementary Fig. 9c, d). Then, we measured CD19 protein surface expression using CD19 antibody staining and flow cytometry analysis (Supplementary Fig. 9e). Strikingly, we found that both cell lines show reduced CD19 surface exposure upon PTBP1 depletion (Fig. 6d–f, Supplementary Fig. 9f). Thus, by interfering with CD19 protein expression on the cell surface, PTBP1 depletion could indeed contribute to CART-19 therapy resistance.
Taken together, our data suggest that both cis-acting mutations and trans-acting RBPs can lead to unproductive CD19 splicing which in turn disrupts CD19 epitope presentation. Therefore, the splicing-affecting mutations and RBP regulators identified in this work may harbour predictive information for CART-19 therapy success.
Discussion
Massively parallel reporter assays such as our high-throughput mutagenesis screen provide comprehensive insights into the regulatory code of splicing, as they characterise the complete set of cis-acting sequence mutations and reveal the binding sites of trans-acting RNA-binding proteins (e.g.,19,20,21,36,37,38). The interpretation of these datasets is challenging due to nonlinear interactions of individual mutation effects. For instance, competition effects in splicing reduce the impact of individual mutations at low and high isoform frequencies, i.e., depending on the mutational background19,20. In addition, other factors such as RBP expression patterns and cell type/tissue identity determine the effects of sequence mutations. Using kinetic modelling, we and others derived regression models taking competition in splicing into account, thereby showing that the effects of complex mutation combinations can be quantitatively described as the sum of individual mutation effects19,20. Thus, mutations seem to control splicing additively rather than synergistically, and this principle also holds for CD19 splicing.
In our CD19 mutagenesis dataset, we comprehensively characterise the full set of splice isoforms generated in response to thousands of sequence mutations. In particular, we find that cryptic splice site activation and thus alternative 3′ and 5′ splice site usage are common modes of alternative splicing. Intriguingly, such events do not require extensive sequence remodelling, but can often be triggered by single point mutations, as indicated by strong associations between putative cryptic isoforms and certain nucleotide substitutions. This suggests, in accordance with previous reports39, that neighbouring splice sites frequently compete for spliceosome assembly, especially if the canonical splice site is comparably weak. While this finding shows the enormous isoform complexity that can arise already from such a simple exon configuration, it raises the question of how protein function can be robustly maintained, since most cryptic CD19 splicing isoforms likely encode non-functional proteins.
Unlike previous mutagenesis screens which mainly focused on exonic sequence mutations, the present CD19 dataset characterises the complete set of intronic and exonic mutations in a 1200 nt sequence stretch. The complete characterisation of CD19 exons 1–3 required the use of long-read sequencing technology. Given that introns in human protein-coding genes on average span ~8.1 kb (GENCODE v31), the long-read sequencing methodology described in this work opens the approach for broad applications. For CD19, we find that strong mutation effects are mainly centred around canonical and cryptic splice sites, whereas in other examples such as MST1R exon 11 or FAS exon 6, mutation effects are more dispersed across intronic and exonic sequences19,40. This suggests that CD19 exon 2 splicing may be controlled by multiple splicing enhancers that act redundantly and render inclusion less sensitive to individual point mutations20. Therefore, CD19 exon 2 may require more specific perturbations and as we show here, does not only respond with exon skipping, but tends to employ alternative splice sites and intron retention, both of which are clinically relevant in the case of CART-19 therapy resistance.
Our retrospective analyses of clinical B-ALL samples implicate unproductive CD19 splice isoforms in the development of CART-19 therapy resistance. Using minigene assays, we directly show that CD19 mutations that are observed in relapsed patients lead to exon 2 skipping, intron 2 retention or an additional isoform that uses an alternative 3′ splice site in exon 2. Furthermore, based on our mutational scan, we report ~200 additional point mutations that significantly affect these and other therapy-impacting isoforms. Thus, our results indicate that far more CD19 mutations can create isoforms that would escape CART-19 recognition. In the future, targeted CRISPR/Cas9 replacement experiments using the endogenous CD19 gene should be performed to validate that the predicted mutations cause physiological changes in splicing, loss of CD19 protein exposure on cell surface and CART-19 therapy resistance. Furthermore, the detection of such mutations in longitudinal samples may provide predictive biomarkers for therapy response in the future.
Likewise, alterations in the expression of trans-acting RBPs can induce aberrant CD19 splicing, explaining the emergence of CD19-negative relapses in samples without mutations or with low-allelic-frequency mutations or without mutations in the CD19 locus. Interestingly, we find that the differentiation status of B cells affects CD19 splicing: in mature B cells, almost complete exon 2 inclusion occurs, implying that all CD19 transcripts give rise to functional CD19 protein. In contrast, intron 2 retention occurs in approximately half of the CD19 transcripts in undifferentiated B-cell precursors (Fig. 1d). Likewise, retention of intron 2 is predominant in B-ALL patient samples from the TARGET B-ALL cohort, with 93% of patients exhibiting retention frequencies above 50% (Supplementary Fig. 1b). Hence, incomplete B-cell differentiation in B-ALL may induce a transcriptional and posttranscriptional programme, likely involving altered RBP expression, that reduces (but does not completely eliminate) the functional CD19 protein pool. This partial intron 2 retention may predispose the cancer cells to therapy resistance before they are actually subjected to CART-19 treatment, as observed in sorted B-cell populations from a B-ALL patients before and after CART-19 therapy relapse17. For the development of complete CART-19 resistance, some B-ALL patients thus likely host subclonal CD19-negative B-ALL cells which are further selected under the treatment17. The causes of complete CD19 loss in these subclonal cell populations are likely to be manifold, involving (epi)genetic changes such as hypermethylation of the CD19 promoter41, mutations in the CD19 gene, splicing factor expression and combinations thereof.
Mutations in splicing factors such as SRSF2, SF3B1 and U2AF1 are common in myelodysplastic syndrome/acute myelogenous leukemia42 and chronic lymphocytic leukemia43, and are associated with aberrant splicing. In B-ALL, mutations in splicing factors are not common, but previous work suggests that splicing factor expression is deregulated44. In the context of CD19, we confirm that SRSF3 deregulation induces exon 2 skipping9 and identify several other RBPs that promote the expression CD19 protein isoforms invisible to the immunotherapeutic agent, including PTBP1, PCBP2, SF3B4, HNRNPK, MBNL1 and HNRNPM. Several of the newly identified regulators have been found as deregulated in other cancer types and are discussed as potential targets for anti-cancer therapy45,46,47. In addition, upregulation of PTBP1 has been implicated in acquired resistance to the chemotherapeutic agent gemcitabine in pancreatic ductal carcinoma cells48. In the context of lymphocytes, PTBP1 is upregulated in B cells and required for early B-cell selection49. It was reported, however, that treatment of leukemic cells with the targeted therapy drug imatinib, which inactivates the BCR-ABL kinase encoded by the translocated Philadelphia (Ph) chromosome, lowers PTBP1 levels50. In the light of our finding that PTBP1 knockdown increases CD19 intron 2 retention and thereby reduces CD19 epitope presentation, previous treatments with imatinib may have negative impact on the subsequent response to the CART-19 therapy in a subset of Ph+ B-ALL patients. In addition, a recent study showed that the repeat RNA PNCTR sequesters substantial amounts of nuclear PTBP1 in various cancers51. Thus, in addition to regulation of PTBP1 expression, other factors such as availability may also influence PTBP1-mediated regulation in B-ALL cells under CART-19 therapy.
Currently, we cannot predict which patients with a CD19-positive B-ALL have a high risk of developing CD19-negative relapses. The pre-existence of isoforms skipping exon 2 or exons 5–6 has been previously discussed as a possible biomarker16,17. Moreover, in a comparison of B cells from a B-ALL patient, it was found that intron 2 retention had already occurred prior to CART-19 therapy (CD19-positive B cells) and had become predominant in the CD19-negative B cells after relapse17. Our results point to the need to extend the analysis to additional CD19 isoforms and to incorporate the expression of splicing factors in screening approaches to identify patients at risk of relapse on CART-19 therapy. Notably, the same biomarkers might also be relevant for other malignancies arising from B-cell lineage, such as large B-cell lymphoma. Loss of CD19 following CART-19 therapy has been described as a mechanism for relapse52, accounting for 60% of relapses in recent clinical studies53. Our data show that CD19 splicing is highly complex, with already ~100 alternative isoforms concerning just exons 1–3. Of them, ~80% encode for a CD19 protein lacking a functional CART-19 epitope and are thus expected to contribute to therapy resistance. The specific detection of alternative splicing might serve as a reliable biomarker and may provide a novel approach to monitor disease progression as already suggested in other tumour entities54. To assess the role of the predicted cryptic splice isoforms in patients, we screened sequencing data from the TARGET B-ALL cohort and indeed recurrently found two junctions from the cryptic isoforms that we had observed in the mutagenesis data. Even though other cryptic junctions were absent and mutations associated with cryptic isoforms according to screen were also not found in the patient data, these may still emerge during CART-19 selection. Currently, there is a shortage of large-scale sequencing data of patient material before and after CART-19 therapy55. Future analysis of such data with a special focus on cryptic splice site usage will be important to identify mutations or splice isoforms that are predictive for CART-19 therapy success.
The contribution of aberrant splicing to CART-19 resistance may further be relevant for future combination therapies. Small-molecule splicing modulators are currently in clinical trials for myeloid neoplasms and splice-switching antisense oligonucleotides are in development for different targets (reviewed in12). Our mutagenesis dataset provides a strong basis for designing and systematically evaluating splice-switching oligonucleotides for the modulation of CD19 splicing. The combined application of these splicing modulators with immunotherapy may represent a way to limit the generation of resistance to CART therapies.
Methods
Cell lines
NALM-6 cells were obtained from ATCC and cultured in RPMI medium (Life Technologies) with 10% fetal bovine serum (Life Technologies) and 1% L-glutamine (Life Technologies). HEK293T cells were obtained from DSMZ and grown with the same additives as for NALM-6. For validation experiments (Fig. 3e), HEK293 cells were obtained from DSMZ and were cultured in Gibco Dulbecco’s Modified Eagle Medium (DMEM, Thermo Fisher Scientific) with L-Glutamine + 10% Gibco foetal bovine serum (FBS, Thermo Fisher Scientific). All cells were kept at 37 °C in a humidified incubator containing 5% CO2. They were routinely tested for mycoplasma infection.
Cloning
The CD19 minigene was amplified from human genomic DNA (Promega) with the primers 5′-catAAGCTTgaccaccgccttcctctctg-3′ and 5′-catGAATTCNNNNNNNNNNNNNNNGGATCCttcccggcatctccccagtc-3′. pcDNA3.1 was used as the vector backbone for the CD19 minigene plasmid. Both the backbone as well as the minigene amplicons were digested with the restriction enzymes EcoRI and HindIII (New England Biolabs). The backbone was extracted from a 1% agarose gel using QIAquick Gel Extraction Kit (Qiagen) and the minigene insert was cleaned up using QIAquick PCR Purification Kit (Qiagen). Ligation was conducted overnight at 16 °C with T4 DNA Ligase (New England Biolabs). All minigene mutations were introduced via Q5 Site-Directed Mutagenesis Kit (New England Biolabs). Position 748 (nucleotide 6 of intron 2) was exchanged from G to T to raise the baseline level of exon 2 inclusion in the WT CD19 minigene to a similar level as in the endogenous CD19 gene. The nine mutations from eight patients in Orlando et al.5 listed in Supplementary Table 1 were inserted into the WT CD19 minigene. For validation experiments (Fig. 3e), 19 individual point mutations with predicted effects on at least one isoform were inserted into a CD19 minigene variant that additionally contained the mutation G742C to adjust the baseline of splice isoforms in HEK293 cells to the pattern seen in NALM-6 cells. All kits were used according to the manufacturers’ recommendations.
Mutagenesis of minigene and library construction
For the random mutagenesis of the CD19 minigene, GeneMorph II Random Mutagenesis Kit (Agilent) was used according to manufacturer’s recommendations using 500 ng CD19 minigene for 30 cycles at 56 °C with the amplification primers 5′-catAAGCTTgaccaccgccttcctctctg-3′ and 5′-catGAATTCNNNNNNNNNNNNNNNGGATCCttcccggcatctccccagtc-3′. PCR products were purified using QIAquick Gel Extraction Kit (Qiagen), digested with EcoRI and HindIII (New England Biolabs) and then ligated into the backbone.
Transfection with minigenes
Cells were twice washed in Dulbecco’s phosphate-buffered saline (DPBS, Gibco Thermo Fisher Scientific) and then collected in R buffer with a density of 2 × 107 cells/ml. For electroporation, we used 5 µg plasmid DNA (with a concentration of at least 1 µg/µl) to 2 × 106 cells in R buffer for a 100 µl NEON electroporation pipette tip (Thermo Fisher Scientific) at 1600 V for 30 ms and 1 pulse. Cells were harvested 24 h later. For validation experiments (Fig. 3e), 7 × 105 cells per well were seeded in six-well TC plates one day prior to transfection. 24 h later, cells were transfected with a mixture of 2 µg plasmid DNA and 20 µg linear Polyethylenimine MW 2500 (PEI 2500, Polysciences), and Gibco Opti-MEM (Thermo Fisher Scientific) was added to 100 µl total volume. This mixture was added dropwise to 1,9 ml fresh DMEM covering the cells, followed by incubation for 24 h.
Quantification of splicing isoforms using semiquantitative RT-PCR
Semiquantitative RT-PCR was used to quantify ratios of CD19 mRNA isoform variants. To this end, reverse transcription was performed on 500 ng RNA with RevertAid Reverse Transcriptase (Thermo Fisher Scientific) according to the manufacturer’s recommendations. Subsequently, 1 μl of the cDNA was used as template for the RT-PCR reaction with OneTaq DNA Polymerase (New England Biolabs). PCRs were run at the following conditions: 94 °C for 30 s, 28 cycles (minigene) or 34 cycles (endogenous CD19) of [94 °C for 20 s, 55 °C for 30 s, 68 °C for 30 s] and final extension at 68 °C for 5 min. The primers 5′-ACCTCCTCGCCTCCTCTTCTTC-3′ and 5′-GCAACTAGAAGGCACAGTCG-3′ were used for the CD19 minigene, and 5′-ACCTCCTCGCCTCCTCTTCTTC-3′ and 5′-CCGAAACATTCCACCGGAACAGC-3′ for the endogenous CD19 gene. A TapeStation 2200 capillary gel electrophoresis instrument (Agilent) was used for quantification of the PCR products on D1000 tapes.
For the semiquantitative RT-PCR experiments in HEK293 cells, cells were harvested 24 h after transfection and pelleted. RNA was isolated using the QiaGen RNeasy kit following the manufacturer’s protocol with the exception of adding only 100 µl of cell lysate onto the gDNA removal columns to ensure proper removal of genomic and/or plasmid DNA. 1–2 µg RNA per sample were used to generate cDNA with the ThermoScientific RevertAid cDNA kit. We changed the second temperature step of the manufacturer’s synthesis protocol from 4 °C to 25 °C (5 min) to further reduce RNA dimerisation or formation of secondary structures. Subsequently, 1 μl of cDNA was used as template for the RT-PCR reaction with OneTaq DNA Polymerase (New England Biolabs). PCRs were run at the following conditions: 94 °C for 30 s, 28 cycles of [94 °C for 20 s, 52 °C for 30 s, 68 °C for 30 s] (minigene) or 34 cycles of [94 °C for 20 s, 55 °C for 30 s, 68 °C for 30 s] (endogenous CD19) and final extension at 68 °C for 5 min. The primers 5′-ACCTCCTCGCCTCCTCTTCTTC-3′ and 5′-GCAACTAGAAGGCACAGTCG-3′ were used for the CD19 minigene, and 5′-ACCTCCTCGCCTCCTCTTCTTC-3′ and 5′-CCGAAACATTCCACCGGAACAGC-3′ for the endogenous CD19 gene. The PCR products were quantified using the TapeStation 4200 system and the High Sensitivity D1000 reagents and tapes (Agilent) according to the manufacturer’s protocol.
Significance of differences in isoform abundance for comparing WT minigenes vs. mutated variants (Fig. 1i) or RBP knockdown vs. control (Fig. 5f) was calculated by a Student’s t test separately for each isoform, reporting the smallest P value for each comparison. A one-way ANOVA was used to test whether isoform abundances are different in any of the three conditions shown in Fig. 1g.
Generation of stable and inducible shRNA knockdown cell lines
Production and preparation of lentivirus
Oligonucleotides with shRNA inserts against eleven RBPs (Supplementary Table 2) were ordered as Ultramer DNA Oligos from Integrated DNA Technologies (Leuven, Belgium). All sequences were based on56. Oligonucleotides containing shRNA inserts were PCR-amplified with primers 5′-TCTCGAATTCTAGCCCCTTGAAGTCCGAGGCAGTAGGC-3′ and 5′-TGAACTCGAGAAGGTATATTGCTGTTGACAGTGAGCG-3′ and purified with QIAquick PCR Purification Kit (Qiagen). shRNA inserts and miRE18_LT3GEPIR_Ren714 backbone (inducible via Tet-On system) were cut with EcoRI and XhoI (New England Biolabs). Backbone was purified from agarose gel with QIAquick Gel Extraction Kit (Qiagen). The fragments were then ligated with T4 DNA Ligase (New England Biolabs) at 16 °C overnight.
Constructs were transduced into NALM-6 via HEK293T-produced lentiviruses. To this end, 10 cm dishes of HEK293T were transfected using 30 µl Lipofectamine 2000 (Thermo Fisher Scientific) with three plasmids: 4 µg shRNA-producing constructs + 2 µg psPAX2 (lentiviral packaging) + 1 µg pMD2.G (lentiviral envelope) at 72 h prior to transduction. On the first day after transfection, the medium was changed. Work with cells used for lentiviral production was conducted in the S2 laboratory.
Transduction of NALM-6 cells
Lentiviral production was confirmed with Lenti-X GoStix (Takara) and lentiviruses were concentrated with Lenti-X Concentrator (Takara) according to the manufacturer’s recommendations. For transduction, 1 × 106 NALM-6 cells in 500 µl of medium were added to the concentrated virus. 5 µg/ml polybrene (Sigma-Aldrich) was added. The cells were centrifuged at 800 g and 32 °C for 30 min. Cells were then transferred into 6-well plates and cultivated in normal growth medium without antibiotics. Selection was started after 48 h with 0.5 µg/ml puromycin (Thermo Fisher Scientific). Antibiotic medium was exchanged every 2–3 days. As soon as cells were not dying under selection anymore and the population was stable, induction experiments were started. After transduction, cells remained in the S2 laboratory for at least 6 weeks. Then, Lenti-X GoStix was used to check for any remaining lentivirus.
Induction of stable shRNA-expressing NALM-6 cells
Controlled by the Tet-responsive TRE3G promoter, the expression of shRNA was induced by addition of doxycycline (Thermo Fisher Scientific). To this end, 2 × 106 NALM-6 cells were seeded into a six-well plate in 2 ml medium containing 0.5 μg/ml puromycin and induced with 0.5 μg/ml doxycycline, diluted in RPMI 1640 medium (Thermo Fisher Scientific). Induction was conducted at 37 °C and 5% CO2 and cells were harvested after 48 h. During induction, the shRNA expression system is coupled to the production of eGFP, which was examined by fluorescence microscopy before harvesting.
Quantitative real-time PCR (qPCR)
RNA was extracted from the induced harvested cells using the RNeasy Plus Mini Kit (Qiagen). This RNA was used for qPCR to validate the RBP knockdown as well as for semiquantitative RT-PCR experiments to check the splicing pattern of endogenous CD19. The qPCR was conducted using the Luminaris HiGreen qPCR Master Mix, low ROX (Thermo Fisher Scientific) according to the manufacturer’s recommendations. Oligonucleotide sequences of all qPCR primers are given in Supplementary Table 3.
Targeted DNA sequencing
DNA-seq of the minigene library was performed on the PacBio SMRT sequencing platform at MPI-CBG Dresden. For this purpose, the minigene plasmid library was digested with EcoRI and HindIII (New England Biolabs) and run on an agarose gel. The desired band at the size of 1301 nt was cut out and purified using QIAquick Gel Extraction Kit (Qiagen). For the run on the PacBio SMRT cell, standard library preparation was performed.
Targeted RNA sequencing
NALM-6 cells were electroporated with the mutated minigene library (see above). 24 h later cells were harvested and RNA was isolated via the RNeasy Mini Kit (Qiagen). 20 µg isolated RNA was poly-A-selected using Dynabeads Oligo (dT)25 beads (Invitrogen) according to the manufacturer’s recommendations. Reverse transcription was performed on 500 ng poly-A-selected RNA with RevertAid Reverse Transcriptase (Thermo Fisher Scientific) according to the manufacturer’s recommendations. To prevent chimeric amplicons, the RNA-seq libraries were amplified via emulsion PCR57 using the Phusion DNA Polymerase (New England Biolabs). The following primers containing Illumina adaptors were used in the PCR: 5′- CAAGCAGAAGACGGCATACGAGATCGGTCTCGGCATTCCTGCTGAACCGCTCTTCCGATCTNNNNNNNNNNGGAACCTCTAGTGGTGAAGG-3′ (fwd) 5′-AATGATACGGCGACCACCGAGATCTACACTCTTTCCCTACACGACGCTCTTCCGATCTNNNNNNNNNNCCGCCAGTGTGATGGATATC-3′ (rev) under following conditions: 98 °C for 30 s, 25 cycles of [98 °C for 10 s, 63 °C for 20 s, 72 °C for 1 min] and final extension at 72 °C for 5 min. Amplicons were purified using Agencourt AMPure XP beads (Backman Coulter). Purified products were analysed on the TapeStation 2200 capillary gel electrophoresis instrument (Agilent) and quantified using the Qubit assay (Thermo Fisher Scientific). RNA-seq was carried out on the Illumina MiSeq platform using paired-end reads of 350 nt + 250 nt length and a 10% PhiX spike-in to increase sequence complexity.
PTBP1 iCLIP2 experiments
We used the iCLIP2 approach for transcriptome-wide mapping of PTBP1 binding to RNA in NALM-6 cells. iCLIP2 was performed according to our previously published protocol35. Briefly, the iCLIP2 libraries were made from NALM-6 cells grown in RPMI as described above (2 × 106 cells per replicate). To induce protein-RNA crosslinks, the cells were irradiated with 150 mJ/cm2 UV light at 254 nm. Next, PTBP1 protein-RNA complexes were immunoprecipitated using 2 µg of anti-PTBP1 antibody (Santa Cruz, sc-56701). RNase digestion was performed by adding 10 µl of 1/300 or 1/500 diluted RNase I (Ambion) to the sample. RNA purification, reverse transcription and library preparation were done as described in35.
PTBP1 siRNA electroporation in MHHCALL4 and P493-6 cells
The cell lines MHHCALL4 and P493-6 were electroporated with a specific siRNA targeting PTBP1 (TAGCAAGATGATACAATGGTA[dT][dT]; Sigma, sR90) or a Scramble control (D-001810-10-50, Dharmacon) using the Neon Transfection System (Thermo Fisher Scientific). In short, 5 × 105 cells were resuspended in 10 µl of 5 µM siRNA in buffer R and electroporated using the Neon Transfection System 10 µL Kit (MPK1096, Thermo Fisher Scientific) with the following settings: 1700 V, 20 ms, 1 pulse. After electroporation, the cells were cultured in the recommended media for 48 h and collected for CD19 cell surface staining, quantitative real-time PCR and Western blot.
CD19 cell surface staining
In all, 1 × 105 cells were resuspended in 50 µl of PBS, 20% FBS, 1 mM EDTA and 2.5 µl of Human TruStain FcX blocking (422302, BioLegend) and incubated for 20 min. After blocking, 2.5 µl of APC anti-human CD19 antibody (1:20, 982406, BioLegend) was added to the cells and incubated for 30 min. Cells were washed twice with PBS, 20% FBS, 1 mM EDTA and the CD19 staining was measured using the BD Accuri C6 Plus Flow Cytometer instrument (BD Biosciences). Flow cytometry data was analysed with FlowJo (version 10.7.2) software.
Western blot
Cell pellets were resuspended in RIPA buffer with Protease/Phosphatase Inhibitor (1861282, ThermoScientific) and 30 µg of protein were loaded in a 10% pre-cast gel (456-1035, BioRad). Antibodies against CD19 (1:1000, #3574, Cell Signalling), PTBP1 (1:500, sc-56701, Santa Cruz Biotechnology) and β-Actin (1:5000, 8H10D10, Cell Signalling) were used for total protein expression detection. Images were acquired with GBox instrument (Syngene).
Quantitative real-time PCR
RNA was extracted using the Maxwell RSC Instrument (Promega) and the Maxwell® RSC simplyRNA Cells Kit (AS1390, Promega). 0.5 µg or RNA were reverse-transcribed using the SuperScript™ IV Reverse Transcriptase kit (18090010, Invitrogen) following the manufacturer’s protocol. RNA expression was measured using SYBR Green Master MIX (Thermo Fisher Scientific). Quantitative real-time PCR was performed in a QuantStudio™ 7 Pro Real-Time PCR System (Thermo Fisher Scientific) with specific primers (Supplementary Table 3) spanning the exon-exon junctions between exons 2 and 3 (E2E3 1&2), 3 and 4 (E3E4), and 10 and 12 (E10E12) as well as the exon-intron junctions from exon 2 to intron 2 (e2i2), from intron 2 to exon 3 (i2e3).
Re-analysis of RNA-seq data from Orlando et al
We re-analysed RNA-seq data of B-ALL patients at screening and after CART-19 therapy relapse from Orlando et al.5 to quantify intron 2 retention in CD19. Since raw data were not available, we obtained BAM files for the different patients deposited in the Short Read Archive (SRA) under the accession SRP141691. For 10 patients, matched data were available at screening and relapse. We excluded one patient (patient #17) after visual inspection indicating that the submitted data in fact corresponded to DNA-seq rather than RNA-seq data. The data contained the aligned reads mapped to several genes from the immune system including CD19. Using custom scripts, we extracted the sequence of the reads, reformatted them and generated fastq files. We then mapped the fastq files to our minigene sequence using STAR58 (v2.6.1). We used the re-mapped reads to quantify the levels of intron 2 retention in the different samples using the R/Bioconductor package ASpli59 (version 1.12.1).
For the expression analysis of B-ALL patients at screening and after CART-19 therapy relapse, we used the gene read counts provided in Supplementary Data Table 1 of Orlando et al.5. Gene lengths were taken from BiomaRt (version 2.4.21) for the human genome version GRCh37 accessed through the R/Bioconductor package OrgDb (version 3.10.0). Normalisation and RPKM calculations were performed using the R/Bioconductor package edgeR60 (version 3.28.1).
DNA-seq barcode demultiplexing
We obtained the circular consensus sequences (CCS), stored as fastq files. Two rounds of sequencing yielded a total of 337,215 CCS. We kept only reads with a length of 150–1150 nt. We adapted the demultiplexing procedure described in19. In this case, we searched for the 15-nt barcode in the last 50 nt of the read. If the barcode was not found, we searched in the last 50 nt of the reverse complementary strand. We only allowed the recovery of barcodes ranging from 14 to 16 nt, which would account for barcodes containing one nucleotide inserted or deleted. Before proceeding with the variant calling, we determined a cutoff to decide the minimal number of CCS to call variants on. Here, we kept only barcodes supported by at least 4 CCS. In total, we recovered 68.5% of all the demultiplexed barcodes which corresponded to 10,558 different minigenes, closely resembling the ~10,000 minigene clones that were used to generate the library.
DNA-seq mapping and variant calling
We use BLASR61 with the standard parameters to map the demultiplexed minigene sequences to the minigene reference. We performed variant calling in the aligned BAM files using the GATK62 HaplotypeCaller (version 4.0.10) with the parameters --kmer-size 10 --kmer-size 15 --kmer-size 25 --allow-non-unique-kmers-in-ref. We used different k-mer sizes to improve the detection of problematic regions. Mixed barcodes, i.e., barcodes containing two classes of mutations, were removed based on the “penetrance score”, reported as allele frequency (AF) in the GATK vcf output files, such that barcodes with more than 25% variants of low penetrance (AF < 0.8) were discarded. Using this strategy, we were able to recover 100,135 mutations of high quality coming from 10,295 distinct minigenes plus an additional 194 unmutated WT minigenes with distinct barcodes. 57.4% of the mutations appeared in at least ten different minigenes.
RNA-seq barcode demultiplexing
RNA-seq libraries were sequenced on Illumina MiSeq as 350 nt + 250 nt paired-end reads, yielding approximately 23 million reads. We controlled their quality using FastQC (version 0.11.5, https://www.bioinformatics.babraham.ac.uk/projects/fastqc/) and removed bad quality ends of reads using Trimmomatic63 (version 0.36, parameters: SLIDINGWINDOW:6:10 MINLEN:0). After trimming, we filtered for read pairs with a minimal length of 305 nt (read1) and 157 nt (read2) and, as done in Braun et al.19, we used matchLRPatterns() and trimLRPatterns() from the R/Bioconductor package Biostrings to extract the 15-nt barcode in read1 between the two flanking restriction sites (Lpattern = TGCAGAATTC, Rpattern = GGATCC) allowing one mismatch. All read pairs with barcode length between 14 and 16 nt were kept for further processing. Barcode sequences were added to the read names in the fastq file and 5′ ends of reads were trimming (read1: everything until the second anchor sequence GGATCC, read2: the first 12 nt). After identifying and trimming the barcode and other regions, we used Cutadapt64 (version 1.6, parameters: --adaptor=TAGAGGTTCC --overlap=3 --error-rate=0.1 --no-indels --minimum-length=244 --pair-filter=both) to remove remaining primer sequences from read1. Lastly, the barcode information attached to the read names was used to demultiplex all read pairs into individual fastq files for each minigene.
Isoform quantification from RNA-seq data
Only barcodes/minigenes also detected in the DNA-seq library were kept for further analysis. All minigenes with insertions or deletions of 10 or more base pairs were removed from further analysis. For better mapping results, we shortened read1 to at most 260 nt. Read pairs of each minigene were mapped to the respective minigene (including all mutations with penetrance ≥0.8, but excluding insertions and deletions) using STAR58 (version 2.6.1b). An annotation of three isoforms (exon 2 inclusion and skipping, as well as the artefact PCR product Δex2part which lacks an internal fragment of exon 2 due to a reverse transcription artefact65) was provided to STAR during mapping and an --sjdbOverhang of 259 was set. When running STAR, all SAM attributes were written, up to ten mismatches were allowed, soft-clipping was prohibited on both ends of the reads and only uniquely mapping reads were kept for further analysis. BAM files were sorted and indexed using SAMtools66 (version 1.5).
Properly and consistently mapped pairs were used for isoform reconstruction using a custom Perl script. Read pairs were considered properly mapped if they mapped with the right orientation on opposite strands. Read pairs mapped consistently if they either did not overlap or in case of an overlap, agreed in their detected splice junctions. Besides, only read pairs for which both mates exceeded the constitutive exon boundaries by at least 10 nt were used for isoform reconstruction. All other pairs were removed since they did not provide any isoform information. Only minigenes covered by at least 100 read pairs usable for isoform reconstruction were kept for further analysis. For each read pair, the CIGAR strings of the two mates were used to reconstruct their splicing isoform. Regarding the artefact product Δex2part, we combined the eight possible mappings of the missing internal fragment of exon 2 which are possible due to the associated 8-nt repeat sequence65. Only isoforms, which were supported by ≥ 1% of the read pairs and at least two read pairs in at least one minigene, were kept for further analysis.
The analysis described above was done separately for two replicates. All isoforms occurring with a frequency of at least 5% in two or more minigene variants in either of the two replicates were kept as individual isoforms. All other detected isoforms were summarised into a category “discarded”. Isoforms with Δex2part, i.e., excluding the internal intron in exon 2, were combined with their “real” counterparts without Δex2part by merging isoforms that only differed in the exclusion of the internal fragment of exon 2. In total, this leads to a set of 101 individual isoforms.
Estimation of single-mutation effects and splicing-affecting mutations
Since the majority of the minigenes in the dataset exhibit more than one mutation, with a mean of 9.6 mutations per minigene, the splicing-affecting mutations cannot be read out directly from the data. We used multinomial logistic regression to infer the effects of single mutations from combined measurements. The regression is based on hypothetical minigenes containing only one mutation, and on the assumption that mutation effects (log fold-changes compared to WT) add up into combined ones at the levels splice isoform ratios19.
For regression, we focused on the five major isoforms that are already present in the WT minigene (see main text). Therefore, minigenes exhibiting more than 5% cryptic isoforms were removed from the dataset, and for the remaining minigenes the cryptic isoforms were merged into a lumped splicing category which we termed “other”. Thus, six categorical splicing outputs (inclusion, skipping, intron2-retention, alt-exon2, alt-exon3, other) were considered in the regression model, and the probability of each these outputs to be observed was assumed to equal the measured isoform frequencies. The regression was formulated as a softmax regression problem using the LogisticRegression command from the Python package scikit-learn67.
Given the large number of mutations per minigene in the dataset, the regression was prone to overfitting (i.e., mutations with weak effects on splicing were assigned non-zero coefficients to fit random fluctuations in the data; not shown). To avoid this problem, we employed L1 penalisation. The strength of the penalty was optimised by tenfold cross-validation, and the resulting inverse regularisation strength was C = 10 for both replicates.
The goodness of the model in describing the measured combined mutation effects (minigenes) was tested by assessing the correlation between model and data in training and test datasets (Supplementary Fig. 4a). Tenfold cross-validation was performed by once randomly splitting the dataset into ten parts. In ten distinct model evaluations, nine of the data sections were simultaneously for model training, whereas the remaining section served as test data. Therefore, each data point is only once part of the test data, and the mean Pearson correlation coefficient between model prediction and test data was used to assess the model performance. Cross-validation at the final penalisation strength (with the highest correlation between model and test data) showed that the method performs very well in estimating the minigene isoform frequencies of the test dataset (Supplementary Fig. 4b). Since we saw little variability in the prediction power for these ten validation runs, we report the average correlation coefficient in Fig. 3b: The Pearson correlation coefficients between softmax predictions of combined mutation effects and measurements lie for the single isoforms between 0.68-0.95 for the first replicate and between 0.71-0.93 for the second replicate.
The accuracy of the model-predicted single-mutation effects in the softmax regression was assessed by leaving out 56 directly measured single-mutation minigenes (i.e., minigenes bearing only one mutation) from the training data. Since most of these 56 mutations are not splicing-affecting, we focused our analysis on the seven mutations that change the inclusion isoform level beyond two standard deviations of the WT minigene distribution: For each of the seven mutations, we performed multiple softmax fits in which the training data: (i) contained all minigenes not harbouring the mutation of interest, (ii) excluded its single-mutation minigenes, and (iii) comprised varying numbers of combined mutation minigenes containing the mutation. For each mutation occurrence between 1 and 10, we used up to 7 different, randomly chosen combinations of multiple mutated minigenes including the mutation of interest. For each of these models, we generated predictions for the single-mutation effect. The prediction accuracy was assessed by calculating the difference between model and direct single-mutation measurements for a certain mutation occurrence. The standard deviation of the difference between model and data was used as a measure for the model error. We find that a mutation occurrence of 3 leads to an error level equal to two WT standard deviations (calculated based on inclusion levels of all WT minigenes in the first replicate). For higher mutation occurrences, the prediction accuracy does not improve further (Supplementary Fig. 4c).
The final modelling step was to identify splicing-affecting mutations. For this purpose, we adopted an approach analogous to empirical P values, i.e., we compared predicted single-mutation effects to empirical isoform frequency distributions in the WT. Isoform frequencies were measured for 195 and 194 WT minigenes in the two replicates. For each isoform and replicate, we chose the 2.5% and 97.5% quantiles of the respective empirical WT frequency distribution as cutoffs (corresponding to a two-sided 5% cutoff). A mutation was considered to have an effect on a splice isoform if, for both replicates, the frequencies predicted by the model were beyond the respective cutoffs and if the effects were in the same direction.
Splice site characterisation
Splice site usage for a given position represents the frequency of the isoforms using a given splice site in a particular minigene divided by the sum of all isoform frequencies for the same minigene. For Fig. 4a, we used the maximum usage of a particular splice site across all minigenes. The strength of putative splice sites along the minigene was calculated using MaxEnt scores26 in sliding windows of 9 nt or 23-nt to evaluate the corresponding sequences as potential 5′ or 3′ splice sites, respectively. The procedure was repeated for all individual point mutations to assess their potential to create cryptic splice sites. For the calculations, we used the Python implementation of MaxEnt (maxentpy, version 0.0.1, https://github.com/kepbod/maxentpy). We filtered the output by keeping only windows that contained a GU or AG dinucleotide in the positions 4–5 (5′ splice site) or 19-20 (3′ splice site), respectively.
We compared the effects of single-point mutations in our library to predictions by the state-of-the-art deep learning algorithm SpliceAI25. We ran SpliceAI (version 1.3.1) with the default parameters plus masking (-M1), using GENCODE68 (v31) annotation for the human genome version hg38 as a reference. Given that SpliceAI results are reported in terms of a probability of gain or loss of a particular splice site, we assigned the gained splice sites in our cryptic isoforms by comparison to the canonical exon 2 inclusion isoform, such that if a new splice site appears in the cryptic isoform, it is considered as “gained” with respect to the “lost” WT splice site. All splice sites in a cryptic isoform were given the same prevalence score, i.e., the prevalence score of the mutation-isoform pair. To compare the SpliceAI scores for a given splice site gain with our prevalence score (Fig. 4f), we considered the mutations that (i) share the same gain-loss pair of positions in both assays, and (ii) are predicted by SpliceAI to gain of a new splice site (i.e., a cryptic site where score_gain > score_loss) upon a given mutation.
RBP binding site predictions
For the prediction of RBP binding motifs, we used the web versions of the oRNAment28 (http://rnabiology.ircm.qc.ca/oRNAment) and ATtRACT27 (https://attract.cnic.es/) databases to query the minigene sequence for presence of RBP motifs (Supplementary Fig. 7a). From the obtained predictions, we collapsed overlapping binding sites from the same tool and RBP.
We used DeepRiPe30 to predict the potential impact of single-point mutations on RBP binding. To this end, we downloaded the trained models for PAR-CLIP and ENCODE eCLIP data on 159 RBPs available in the GitHub repository (https://github.com/ohlerlab/DeepRiPe). We scored each mutation (annotated with regards to the hg38 reference genome) across the individual RBP models and reported every mutation for which the model score changed by at least 0.1 in either direction compared to the WT sequence (Supplementary Data 6, worksheet “DeepRiPe mutations”). Positive and negative delta scores refer to a predicted increase or reduction in RBP binding, respectively. The scoring functions are based on the iPython notebooks provided by DeepRiPe: https://colab.research.google.com/drive/18yeqRE7KmOjfbUaLAfJ6rMBjAulYo-Uc?usp=sharing
For the definition of significant RBP binding sites, we used the following strategy. For binding sites predicted by oRNAment and ATtRACT, we first checked their overlap separately for each isoform. If a binding site overlapped in at least one position with a splicing-affecting mutation with respect to this particular isoform, we defined this binding site as an isoform-specific significant binding site. All binding sites that were significant for at least one isoform were collapsed into the complete list of significant binding sites, yielding a total of 315 significant binding sites for 74 RBPs. In the case of DeepRiPe, a mutation with a delta score >0.25 for a given RBP model was required to overlap with a splicing-affecting mutation for a particular isoform (our screen) to be considered an isoform-specific significant RBP-changing mutation. In a similar manner, all isoform-specific mutations for any isoform were collapsed into a complete list of significant RBP-changing mutations, yielding a total of 222 significant mutations that affected the binding of 58 RBPs.
iCLIP data processing
iCLIP libraries were sequenced on an Illumina NextSeq 500 sequencing machine as 92 nt single-end reads including a 6 nt sample barcode as well as 5 + 4 nt unique molecular identifiers (UMIs). Basic quality controls were done with FastQC (version 0.11.8) (https://www.bioinformatics.babraham.ac.uk/projects/fastqc/) and reads were filtered based on sequencing qualities (Phred score) in the barcode region using the FASTX-Toolkit (version 0.0.14) (http://hannonlab.cshl.edu/fastx toolkit/) and seqtk (version 1.3) (https://github.com/lh3/seqtk/). Reads were demultiplexed based on the experimental barcode, which is found on positions 6 to 11 of the reads, using Flexbar69 (version 3.4.0). Afterwards, barcode regions and adaptor sequences were trimmed from read ends using Flexbar. Here, a minimal overlap of 1 nt of read and adapter was required, UMIs were added to the read names and reads shorter than 15-nt were removed from further analysis. Downstream analysis was done as described in Chapters 3.4 and 4.1 of Busch et al.70. Genome assembly and annotation of GENCODE68 v31 were used during mapping.
Patient data analysis
RNA-seq data of 222 B-ALL patients from the Therapeutically Applicable Research To Generate Effective Treatments (TARGET) programme (https://ocg.cancer.gov/programs/target) were processed from fastq files. Sequencing adaptors were trimmed with TrimGalore71 (version 0.6.6), aligned to the hg38 human genome assembly with STAR58 (version 2.5.2a), and sorted and indexed with SAMtools66 (version 1.11). Splice junctions were quantified individually for each sample using MAJIQ72 (version 2.2) and ENSEMBL reference transcriptome GRCh38.9473. Only splice junctions with a usage level (percent selected index, PSI) of at least 5% in any given TARGET B-ALL samples were quantified. The local splicing variation (LSV) harbouring alternative splicing in the region of the CD19 minigene (Supplementary Fig. 1a) was quantified in 220 out of 222 B-ALL patients. For comparison, we used RNA-seq data of immature and mature B cells from healthy donors from44,74.
Annotated variant call format (VCF) files were downloaded for the TARGET B-ALL patient cohort from the NCI Genomic Data Commons (GDC) Data Portal (accessed 11/18/2021). These files are available under controlled access (see Acknowledgements). In brief, the VCF files had been generated from patient whole-exome DNA-seq data using the GDC DNA-seq Analysis Pipeline (https://docs.gdc.cancer.gov/Data/Bioinformatics_Pipelines/DNA_Seq_Variant_Calling_Pipeline/) which includes genomic alignment with BWA, data clean-up with Picard tools and GATK, and calling of somatic variants from matched samples of tumor and adjacent normal tissue for each patient with Mutect2. The raw VCF files were further annotated using the Variant Effect Predictor (VEP) tool to infer the location of each mutation, its consequence (frameshift/silent mutation) and the affected gene(s) as well its overlap with known variants in databases such as ClinVar and dbSNP. Using custom scripts, a total of 468 VCF files of TARGET B-ALL patients were parsed for CD19 mutations. This identified 39 patients with somatic mutations within the CD19 gene, including 11 mutations in the CD19 minigene region (Supplementary Data 4).
Reporting summary
Further information on research design is available in the Nature Research Reporting Summary linked to this article.
Data availability
The sequencing data generated in this study have been deposited in the Gene Expression Omnibus (GEO) database under accession code GSE182894. The collection consists of the PacBio DNA-seq libraries (GSE182892) [https://www.ncbi.nlm.nih.gov/geo/query/acc.cgi?acc=GSE182891], the Illumina RNA-seq libraries (GSE182892) and the PTBP1 iCLIP2 libraries in NALM-6 cells (GSE182893). The results published here are in whole or part based upon data generated by the Therapeutically Applicable Research to Generate Effective Treatments (https://ocg.cancer.gov/programs/target) initiative, phs000218. The data used for this analysis are available at https://portal.gdc.cancer.gov/projects. The remaining data are available within the Article, Supplementary Information or Source Data files. Source data are provided in this paper.
Code availability
The computational code for the analyses and figure generation is available in Zenodo [https://doi.org/10.5281/zenodo.6614454]/Github [https://github.com/mcortes-lopez/CD19_splicing_mutagenesis] under an open-source MIT license.
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Acknowledgements
The authors would like to thank the members of the participating labs for their support and discussion. We would like to thank Sylvia Weiss, Dpt. Systems Biology, University of Stuttgart for technical assistance. We gratefully acknowledge the Institute of Molecular Biology Core Facilities for their support, especially the Genomics Core Facility and the use of its NextSeq 500 (funded by the Deutsche Forschungsgemeinschaft [DFG, German Research Foundation] INST 247/870-1 FUGG) and the Bioinformatics Core Facility. We gratefully acknowledge the PacBio SMRT sequencing platform at MPI-CBG Dresden. TARGET data used for the analyses were accessed under dbGaP project #10088: “Alternative splicing in pediatric cancers”, sub-studies phs000463.v21.p8 and phs000464.v21.p8 (Acute Lymphoblastic Leukemia (ALL) Pilot Phase 1 and Expansion Phase 2). This work was funded by the Naturwissenschaftlich-Medizinische Forschungszentrum (NMFZ) to J.F., J. K. and C. P. and the Deutsche Forschungsgemeinschaft (DFG) to K.Z., J.K. and S. L. (ZA 881/2–3 to K. Z., KO 4566/4-3 to J. K., and LE 3473/2–3 to S. L.). K. Z. was also supported by the Deutsche Forschungsgemeinschaft (SFB902 B13). This work was supported by the grant from the National Institutes of Health (U01 CA232563 to A. T.-T. and Y. B.), St. Baldrick’s-Stand Up to Cancer (SU2C-AACR-DT-27-17 to A. T.-T.) and the V Foundation for Cancer Research (T2018-014 to A. T.-T.). M. T. D. acknowledges support from The Ellen Weisberg Fund: Advancing Breakthroughs in Pediatric Cancer.
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M.C.-L. performed most bioinformatics analyses. L. S. performed the CD19 minigene experiments as well as the massively parallel CD19 splicing reporter assay. L.S. and B.S performed shRNA-mediated RBP knockdown experiments and corresponding splicing assays. M.M. and M.M.M. helped with experiments. M.E. and S.L. designed the mathematical modelling and prevalence score approach, and M.E. performed the analyses. F.K. contributed to the quantification of mutation effects. S.U. and M.K. validated single-mutation effects from model predictions. A.O., M.C.-L., L.S. and J.K. performed PTB iCLIP experiments. M.T.D. performed CD19 flow cytometry assays upon PTBP1 knockdown and associated measurements. A.B. performed iCLIP and RNA-seq data processing as well as splice isoform quantification. M.Q.-V., M.T.D. and R.S. performed TARGET ALL data analysis under supervision of Y.B. and A.T.-T.. Study was designed by M.C.-L., L.S., M.E., K.Z., S.L. and J.K. with help from C.P., J.F. and all co-authors. K.Z., S.L. and J.K. supervised most of the bioinformatics analyses, mathematical modelling, and experimental work, respectively. M.C.-L., L.S., M.E., C.P., K.Z., S.L., and J.K. wrote the manuscript with help and comments from all co-authors.
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A.T.-T. has an interest in intellectual property “Discovery of CD19 Spliced Isoforms Resistant to CART-19”. This interest does not meet the definition of a reviewable interest under Children’s Hospital of Philadelphia’s (CHOP’s) conflict of interest policy and is therefore not a financial conflict of interest. Furthermore, this intellectual property has not been licensed or otherwise commercialised to date. However, should this technology be commercialised in the future, A.T.-T. would be entitled to a share of royalties earned by CHOP per its patent policy. The other authors have no competing interests.
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Cortés-López, M., Schulz, L., Enculescu, M. et al. High-throughput mutagenesis identifies mutations and RNA-binding proteins controlling CD19 splicing and CART-19 therapy resistance. Nat Commun 13, 5570 (2022). https://doi.org/10.1038/s41467-022-31818-y
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DOI: https://doi.org/10.1038/s41467-022-31818-y