The autophagy scaffold protein ALFY is critical for the granulocytic differentiation of AML cells

Acute myeloid leukemia (AML) is a malignancy of myeloid progenitor cells that are blocked in differentiation. Acute promyelocytic leukemia (APL) is a rare form of AML, which generally presents with a t(15;17) translocation causing expression of the fusion protein PML-RARA. Pharmacological doses of all-trans retinoic acid (ATRA) induce granulocytic differentiation of APL cells leading to cure rates of >80% if combined with conventional chemotherapy. Autophagy is a lysosomal degradation pathway for the removal of cytoplasmic content and recycling of macromolecules. ATRA induces autophagy in ATRA-sensitive AML and APL cells and autophagy inhibition attenuates ATRA-triggered differentiation. In this study, we aimed at identifying if the autophagy-linked FYVE-domain containing protein (ALFY/WDFY3) is involved in autophagic degradation of protein aggregates contributes to ATRA therapy-induced autophagy. We found that ALFY mRNA levels increase significantly during the course of ATRA-induced differentiation of APL and AML cell lines. Importantly ALFY depletion impairs ATRA-triggered granulocytic differentiation of these cells. In agreement with its function in aggrephagy, knockdown of ALFY results in reduced ATRA-induced proteolysis. Our data further suggest that PML-RARα is an autophagy substrate degraded with the help of ALFY. In summary, we present a crucial role for ALFY in retinoid triggered maturation of AML cells.

emphasized that degradation of PML-RARα is deemed to be a key event in the elimination of LICs, which is the pre-requisite for a long-term cure of APL 10 . Several pathways are implicated in the ATRA-dependent degradation of PML-RARα, such as direct targeting by caspases and proteosomal degradation 11,12 . A role for autophagy in ATRA-induced degradation of PML-RARα has recently been established 13,14 . Indeed, inhibition of autophagy by pharmacological agents reduces ATRA-induced granulocytic differentiation of APL cells 13 . Similarly to PML-RARα, leukemic oncofusion proteins such as BCR-ABL and FLT3-ITD are subjected to autophagic degradation during targeted therapies 15 .
Autophagy is a process that leads to the degradation of cytoplasmic constituents in the lysosomal compartment. Depending on how the cargo enters the lysosome, three types of autophagy can be distinguished: Macroautophagy, chaperone-mediate autophagy and microphagy 16 . Macroautophagy (hereafter referred to as autophagy) involves the formation of a double membrane structure, the so called autophagosome, which finally fuses with the lysosome to degrade its content. The process of autophagy is executed by numerous autophagy related genes (ATGs), whose encoded proteins generate the autophagosome in an orchestrated manner 17 . Depending on the substrate macroautophagy can be further subdivided in distinct sub-processes. For instance, aggrephagy is the selective removal of aggregated proteins, which tend to accumulate in the cytoplasm and disturb the proper cellular function 18 . The principle of selective degradation by autophagy relies on the presence of a ligand, which specifically targets the cargo for degradation. Recognition of the ligand by an autophagy receptor enables interaction with the autophagy machinery and mediates cargo degradation. Autophagy scaffold proteins assist autophagy receptor proteins and serve as platforms to facilitate the interaction between the receptor targeted cargo and the autophagy machinery 19 . A well-known autophagy receptor is p62, which mediates the degradation of various ubiquitinated cargos including damaged mitochondria, protein aggregates and microbes 20 . Interestingly, p62 supports autophagy-dependent PML-RARα degradation 14 .
Autophagy-linked FYVE-domain containing protein (ALFY/WDFY3) is an autophagy scaffold protein and was originally identified as a PI3P interacting protein localizing to autophagic membranes 21 . Upon autophagy-induction, ALFY translocates from the nucleus to the cytoplasm where it assists p62 in the autophagy-dependent degradation of ubiqutinated protein aggregates in neurodegenerative diseases 22,23 . ALFY interacts with ATG5 in a protein complex consisting of ATG12, ATG5 and ATG16L 24 , supporting the notion that ALFY is an autophagy scaffold protein 25 . In line with this hypothesis, Lystad et al. 26 identified a LC3-interacting region (LIR) in ALFY. The LIR is likely to mediate the interactions with different ATG8 family members. All this prompted us to investigate the role of ALFY in myeloid differentiation and aggrephagy.

Results
ALFY is upregulated during ATRA-induced differentiation of AML cells. In order to establish a role for ALFY in the granulocytic differentiation of AML cells, we exposed NB4 and HT93 APL as well as HL60 AML cells to ATRA for different amounts of time. In NB4 cells, ATRA exposure led to a 5.7-and 30.6-fold up-regulation of ALFY mRNA levels at day 4 and 6, respectively (Fig. 1a). A similar ALFY mRNA induction was observed in ATRA treated HT93 (Fig. 1b) and HL60 (Fig. 1c) cells. To support the idea that ATRA-triggered induction of ALFY mRNA is dependent on granulocytic differentiation, similar experiments were performed in the ATRAresistant sub-clones NB4-R2 and HL60-R2. In both cell lines, no significant modification in the levels of ALFY mRNA was observed ( Fig. 1a and c). Taken together, our data indicate that ALFY mRNA is upregulated only in AML cells, which undergo granulocytic differentiation upon exposure to ATRA. To evaluate whether ALFY is functionally involved in APL differentiation, we inhibited granulocyte maturation by knocking down the key myeloid transcription factors, PU.1 and CEBPα 27 . Knock-down efficiencies are shown in supplementary Figure 1. As expected, inhibition of these transcription factors resulted in reduced levels of differentiation, as indicated by lower mRNA levels of the well-established granulocyte differentiation marker CEBPE (Supplementary Figure 1). These effects were accompanied by a significant impairment of ALFY upregulation (Fig. 1d,e). The results are consistent with the notion that ALFY mRNA levels are upregulated in a PU.1-and CEBPα-dependent manner during APL cell differentiation.
ALFY is down-regulated in primary AML and increases during normal neutrophil differentiation. Since ALFY expression is significantly induced during granulocytic differentiation of AML-derived cell lines, we compared ALFY mRNA levels in AML patients (FAB M0-M4) and granulocytes from healthy donors. The patient characteristics are listed in supplementary Table 1. In line with our findings that ALFY is upregulated in differentiated AML cells, we found significantly lower levels of ALFY in immature blast cells of primary AML patients when compared to mature neutrophils from healthy donors (Fig. 2a). Accordingly, ALFY transcript levels gradually increased during neutrophil differentiation of CD34 + from three healthy donors upon G-CSF treatment (Fig. 2b). In fact, we found a significant upregulation of ALFY mRNA on day 6 of G-CSF stimulation. These data were confirmed by an analysis performed on publicly available data contained in the bloodspot database 28 (Fig. 2c). Taken together, our results suggest an involvement of ALFY not only in ATRA-triggered differentiation of AML cells but also in normal granulocytic maturation.
ALFY is targeted by the oncogenic microRNA miR-181b. To gather information as to the molecular mechanisms underlying ALFY mRNA induction by ATRA, we used the miRWalk prediction database 29 and identified members of the miR-181 family as potential ALFY 3′UTR targeting miRNAs. Since miR-181b is over expressed in promyelocytes from APL patients cells and downregulated during normal and ATRA treated granulocyte development 30,31 , we focused our attention on this miRNA. Indeed, miR-181b specifically inhibited an ALFY 3′UTR reporter construct. In contrast, miR-138, which is not predicted to bind to ALFY 3′UTR, or a scrambled sequence, did not exert any effect on the reporter construct (Fig. 3a). Importantly, ectopic expression of miR-181b caused a significant down-regulation of the basal ALFY mRNA levels in NB4 cells grown under control conditions. The effect was more pronounced in NB4 cells exposed to ATRA (Fig. 3b). In ATRA-treated and miR-181b over-expressing NB4 cells, the down-regulation of ALFY mRNA was accompanied by reduced neutrophil differentiation as shown by a significant reduction in the amounts of mRNA coding for CEBPE (Fig. 3d). In the same experimental conditions we observed a trend towards a decrease in the levels of the CSF3R mRNA, coding for another granulocytic marker (Fig. 3e). Our results are consistent with the idea that miR-181b is a new negative regulator of ALFY mRNA during granulocytic differentiation of NB4 cells.
ALFY significantly contributes to retinoid-mediated differentiation of AML cells. In order to test our hypothesis that ALFY is essential for granulocytic differentiation of APL cells, we generated four NB4-derived cell populations stably expressing three different small hairpin RNAs (shRNAs) constructs targeting ALFY (shALFY1-3) and a control shRNA construct (shC), using lentiviral vectors. The knock-down efficiencies of the three single shRNA constructs as well as the mixture of the corresponding shRNAs (shALFY M) are shown in Fig. 4a. Following exposure to ATRA for 6 days, the differentiation of ALFY-depleted NB4 cells was significantly reduced relative to the respective shC infected control cells, as indicated by the reduced expression of the CEBPE and CSF3R differentiation markers (Fig. 4a). We further established granulocytic differentiation using the nitro blue tetrazolium (NBT) reduction assay. As compared to the corresponding controls, ALFY knock-down caused a significant decrease in the number of NBT-positive cells following 6 days of ATRA exposure (Fig. 4b).
Quantification of the NBT assay from 3 independent experiments indicates that approximately 90% of the control cell population was NBT-positive, while this positivity decreased to 50-70% following ALFY knock-down (Fig. 4c). The results were confirmed in the HT93 cell line (Supplementary Figure S2). To support a role for ALFY in the granulocytic maturation of APL cells, we repeated the experiments using the synthetic retinoid, acitretin, as the compound was previously shown to induce granulocytic differentiation of APL cells both in vitro and in vivo 32 . Furthermore acitretin belongs to a group of retinoids, which induce differentiation but do not cause PML-RARα degradation 32 . Acitretin treatment for 6 days resulted in a strong upregulation of ALFY mRNA in control transduced NB4 cells (Fig. 4d). As observed in the case of ATRA, ALFY depletion significantly reduced acitretin-dependent induction of CEBPE, CSF3R and NBT-positivity ( Fig. 4d-f). As we observed that ATRA causes a significant upregulation of ALFY in the non-APL cell line, HL60 (Fig. 1c), we further assessed granulocytic differentiation in ALFY-depleted HL60 cells. Similar to what was observed in NB4 cells, ALFY knock-down reduced the potential of HL60 cells to undergo granulocytic differentiation upon exposure to ATRA, as assessed by CEBPE and CSF3R mRNA levels (Fig. 4g). In conclusion, our data indicate that ALFY plays a crucial role in retinoid-triggered neutrophil differentiation of AML cells.

NB4 ALFY knock-down cells display reduced proteolysis upon exposure to retinoids. To get
insights into the molecular and cellular processes underlying the action of ALFY on granulocytic differentiation we performed a number of studies in NB4 cells. As ALFY is known to mediate autophagy-dependent degradation of protein aggregates 22 , we measured lysosomal proteolysis under ATRA and acitretin treatment using the long-lived protein degradation assay (LLPDA). As expected ATRA 33 as well as acitretin treated NB4 control cells displayed enhanced proteolysis of long-lived proteins (Fig. 5a). To measure lysosomal degradation, we used bafi-lomycinA1 (BafA), an inhibitor of the vacuolar type H + -ATPase. In fact, BafA inhibits the acidification of lysosomes, suppressing protein degradation 34 . In control transduced cells, BafA partially blocked ATRA-and acitretin induced proteolysis, confirming that the two retinoids induce protein degradation via the lysosomal compartment (Fig. 5a). In contrast, ATRA or acitretin treatment caused only a minor and non-significant increase of protein degradation in ALFY-silenced NB4 cells (Fig. 5a). Importantly, BafA-sensitive and thereby autophagy-dependent  (1)(2)(3) were in vitro differentiated towards granulocytes using G-CSF. ALFY transcript levels were measured at day 0 (d0), day 3 (d3) and day 6 (d6) using qPCR and normalized to HMBS. Friedman test followed by corrected Dunn's post hoc test for multiple comparison was applied. * p < 0.05. (c) The panel displays the results obtained from the "normal haematopoiesis with AMLs" dataset contained in the bloodspot database. Please refer to the website for details on the dataset characteristics. HSC: hematopoietic stem cells, MPP: multipotent progenitors, CMP: common myeloid progenitor, GMP: granulocyte monocyte progenitor, PM: promyelocyte, MM: metamyelocyte, BC: band cell, PMN: polymorph nuclear cells. Kruskall-Wallis test followed by corrected Dunn's post hoc test for multiple comparison was applied. **** p ≤ 0.0001. proteolysis was significantly lower in retinoid treated ALFY knock-down NB4 cells as compared to control transduced cells (Fig. 5b). Of note, basal proteolysis was not affected by ALFY knock-down. Together these results suggest a role for ALFY in retinoid-mediated proteolysis.
Since PML-RARα is degraded via autophagy in a p62 dependent manner 14 , we wondered whether ALFY is involved in this process. To this end, we used HEK293T cells overexpressing PML-RARα to avoid confounding factors generated by the differentiation process activated by ATRA in myeloid cells. Using this model we found ALFY in a complex with PML-RARα in co-immunoprecipitation experiments (Fig. 5c). Moreover, the levels of PML-RARα decreased upon induction of autophagy by serum and amino acid starvation (Fig. 5d). The starvation dependent down-regulation of PML-RARα was however not seen in cells depleted of the core autophagy protein ULK1, confirming its degradation by autophagy. Similarly, depletion of ALFY resulted in higher basal levels of PML-RARα that were not reduced upon starvation (Fig. 5d). ALFY also interacts with PML-RARα in NB4 cells, as endogenous PML-RARα, but not RARα, co-immunoprecipitated with endogenous ALFY (Fig. 5e). These results suggest that PML-RARα is a target for starvation-induced autophagic degradation when over-expressed in HEK293T cells and that ALFY is involved in this process. The participation of ALFY in endogenous PML-RARα degradation in NB4 cells needs further investigation, although it is clear that ALFY knock-down significantly reduces lysosomal degradation upon retinoid exposure.

Discussion
In the present study we found that exposure of AML blasts to ATRA and a derived synthetic retinoid (acitretin) leads to increased expression of the autophagy related gene ALFY. In addition, the knock-down of ALFY decreases or delays the granulocytic differentiation of AML cells. Interestingly, ALFY mRNA was significantly up-regulated during G-CSF-triggered neutrophil differentiation of CD34 + progenitor cells. In accordance with this last finding, ALFY mRNA expression is increased in granulocytes as compared to neutrophil precursors and hematopoietic stem cells. Thus, our data provide evidence for the involvement of ALFY not only in the granulocytic differentiation of AML blasts, but also of normal myeloid cells. Importantly, we demonstrated lower levels of ALFY in AML patients than in mature granulocytes from healthy donors. The observation suggests that the low amounts of ALFY observed in AML are not simply due to deregulated expression of the gene in this disease but they rather reflect the immature myeloid phenotype of the leukemic blasts.
We further investigated how ALFY mRNA is regulated during the granulocytic differentiation of the APL-derived and PML-RARα positive NB4 cell line. In particular, we focused on the potential role of miRNAs in the control of ALFY expression. MiRNAs are small non-coding RNAs regulating mRNA expression. MiRNAs can be oncogenic or tumor suppressive and are often dysregulated in cancer 35 . A recent set of studies has implicated miRNAs in the regulation of autophagy including ATRA-triggered autophagy via targeting of mRNAs controlling different steps of the pathway 36,37 . Here we report that ALFY is yet another autophagy gene regulated by a miRNA in APL cells, i.e. miR-181b. Although we cannot exclude that miR-181b regulates ALFY mRNA indirectly, our data demonstrate that over-expression of miR-181b in NB4 cells leads to down-regulation of the ALFY transcript even under control conditions. The down-regulation of miR-181b in NB4 cells exposed to ATRA 30,31 provides one explanation for the up-regulation of ALFY mRNA during neutrophil differentiation. Interestingly, members of the miR-181 family have been shown to attenuate autophagy via targeting ATG5 under various conditions 38,39 . As ATG5 inhibition exerts a negative impact on neutrophil differentiation of AML cells as well 14 , we propose that the marked inhibitory effects of miR-181b expression on neutrophil differentiation are due to its ability to target more than one ATG gene.
Autophagy is an important homeostatic process taking place in virtually all cells at basal levels that can be further upregulated under stress 40 . It is well established that autophagic flux is activated upon ATRA stimulation of APL cells 13,14,33,41,42 , where it contributes to the degradation of PML-RARα 13,14 . ALFY is an autophagy scaffold protein involved in the degradation of ubiqutinated protein aggregates 21,22 . In agreement with its function in aggrephagy, we found reduced autophagy-dependent proteolysis in retinoid treated ALFY knock-down cells. One potential substrate that is targeted to the autophagosome by ALFY is PML-RARα. Indeed, both ALFY and PML-RARα are part of a complex in HEK293T cells. Furthermore, starvation induced autophagic degradation of ectopic PML-RARα is ALFY dependent, and it is very likely that ALFY also contributes to therapy-induced degradation of PML-RARα in NB4 cells. Importantly, PML-RARα degradation is key to long-term APL remission as it reduces the number of LICs 32 . This emphasizes the importance of developing innovative therapies aiming at degrading PML-RARα. With respect to this, autophagy induction may represent a valid strategy for the treatment of APL since it contributes to PML-RARα degradation at least in vitro 13,14 . Further studies aiming at defining the effects of autophagy induction on PML-RARα levels in LICs, the contribution of ALFY to the process and the impact on the therapeutic effect are of interest.
PML-RARα is unlikely to be the only substrate to be degraded with the assistance of ALFY as it could not fully explain the block in differentiation. In fact, PML-RARα degradation is not required for the granulocytic differentiation of APL blasts, as indicated by studies performed with uncoupling retinoids, a series of compounds which induce differentiation but do not degrade PML-RARα 32 . In addition, PML-RARα stabilization via reduction of its proteasomal degradation enhances the differentiation capacity of ATRA treated APL cells in vitro 43,44 Consistent with these last observations, we demonstrate that the uncoupling retinoid, acitretin, accelerates the maturation process of NB4 cells causing an induction of the neutrophil differentiation markers, CEBPE and CSF3R, as well as the up-regulation of ALFY. Noticeably, ALFY depletion has a negative impact on acitretin-dependent differentiation of NB4 cells. This supports the notion that ALFY controls the degradation of additional proteins during neutrophil differentiation. In line with this hypothesis, our data indicate that ALFY is also crucial for ATRA-triggered granulocytic differentiation of PML-RARα negative HL60 AML cells. Analyzing binding partners of ALFY during neutrophil differentiation of HL60 or CD34 + cells might allow identification of proteins in addition to PML-RARα that need to be degraded for effective differentiation.
During the process of myeloid differentiation and maturation, cells undergo major morphological and homeostatic changes to acquire novel and specific functions. Autophagy might contribute to this process due to its ability to degrade whole organelles as shown for late stage erythroid development where autophagy is involved in removing mitochondria 45,46 . In addition, autophagy plays a crucial role in cell survival during stress conditions by recycling cellular building blocks 47 . Therefore, autophagy could support differentiation by providing metabolic ***P ≤ 0.001. (d) NB4 control (CTRL) or shALFY transduced cells were treated with 1 µM acitretin for 6 days and qPCR analyses were performed to measure ALFY, CEBPE and GC3SFR mRNAs. Raw Ct values were normalized to HMBS and to the untreated control of day 6 (∆∆Ct). Standard deviations were calculated on three independent experiments. (e-f) NBT assays were performed as described in Fig. 2. The percentage of positive cells was calculated from three independent experiments, comparing control and ALFY depleted cells under acitretin treatment at day 6 (g) HL60 control and shALFY transduced cells were treated with 1 µM ATRA and knockdown efficiency as well as differentiation was assessed by measuring ALFY, CEBPE and CSF3R mRNA expression. Normalization was performed as described in A. Mann-Whitney-U test: *P < 0.05, **P ≤ 0.01, ***P ≤ 0.001. Figure 5. ALFY contributes to retinoid-induced lysosomal protein degradation. (a) Control and ALFY knockdown NB4 cells were treated with 1 µM ATRA or acitretin and long-lived protein degradation assays were carried out at day 4. Where indicated, bafilomycinA1 was added to inhibit lysosome dependent protein degradation. Radioactivity was determined by liquid scintillation counting of at least 3 independent experiments. The percentage of total proteolysis is shown. (b) The panel contains the data of the long-lived protein degradation assays as in A. The results are expressed as bafilomycinA1 (BafA) sensitive proteolysis which was calculated by subtracting the value of the BafA treated sample from the corresponding single agent treatment. (c) HEK293Tcells over-expressing PML-RARα were subjected to immunoprecipitation using anti-ALFY or the corresponding IgG antibody as a control. Western blot (WB) analysis of the immunoprecipitated proteins (IP) and of the total cell lysate (TCL) was performed using RARα (to detect PML-RARα at 110 kDa) and ALFY antibodies. Tubulin was used as a loading control. (d) HEK293T cells were transfected with control RNA, ULK1-or ALFY-targeted siRNA followed by transfection with PML-RARA cDNA. The different cell lines were subjected to starvation for 4 hours before western blot analysis of PML-RARα (~110 kDa) was performed. Tubulin is shown as a loading control. (e) The immunoprecipitation of NB4 cell lysates with anti-ALFY or the corresponding IgG antibody is shown. The Immunoprecipitated proteins (IP) and the total cell lysate (TCL) were subjected to western blot analysis for PML-RARα (110 kDa, using RARα antibody), RARα (~50 kDa) and ALFY using Tubulin as a loading control.
substrates. Alternatively it is involved in regulating signalling pathways by selective degradation of signalling molecules 48 . In this context, ALFY could support the degradation of cargo molecules involved in morphological changes or regulating protein signalling levels via aggrephagy. Indeed, ALFY participates in the control of Wnt signalling by removing aggregates of DVL3 via autophagy 49 . Clearly, additional studies are required to support all these hypotheses and to investigate possible non-autophagy related functions of ALFY which may provide information as to its role in AML differentiation.

Generation of knock-down cells.
TaqMan low density array (TLDA) and quantitative PCR (qPCR). RNA extraction was performed using the miRCURY RNA Isolation Kit from Exiqon (Vedbaek, Denmark) according to the manufacturer's instructions. RNA was reverse-transcribed using the masterscript kit purchased from 5prime (Hilden, Germany).
Quantitative PCR analysis of ALFY, CEBPE and CSF3R mRNAs was performed using TaqMan ® reagents and the StepOnePlus qPCR system (Applied Biosystems, Zug, Switzerland). Raw Ct values were normalized to HMBS and to the untreated control of day 4 or 6 (2 −∆∆CT method 52 ). The gene Expression assays for ALFY (Hs00385595_ m1), CEBPE (Hs00797944_s1) and CSF3R (Hs00357657_m1) were ordered at Applied Biosystems (Rotkreuz, Switzerland). The HMBS primers and probes have been described previously 53 . QPCR analysis of ALFY in patients and primary granulocytes was performed using TaqMan Low-Density Arrays (TLDA) using the ABI7500 qPCR assay system (Applied Biosystems, Zug, Switzerland). Raw Ct values were normalized to HMBS and ABL-1 (∆Ct). TLDA measurements as well as data analysis were performed as described 54 . NBT assay. Cells were stimulated for 10 minutes with 200ng/ml phorbol myristate acetate (PMA) in the presence of 1 mg/ml NBT. Both reagents were purchased from Sigma-Aldrich (Buchs, Switzerland). Cells were fixed using CytoSpin and counterstained with Safranin (0.25 g safranin/50 ml dissolved in 20% ethanol). Quantification of the NBT assays was performed by counting the percentage of NBT positive cells. Differences in colour intensity were not considered.
Quantitative PCR of microRNAs. Isolation of microRNAs was performed using the miRCURY ™ Isolation Kit from Exiqon (Vedbaek, Denmark). Expression levels were determined using the miRCURY LNA ™ universal RT microRNA PCR kit (Exiqon, Vedbaek, Denmark) according to manufacturer's instructions. Raw C t values were calculated according to the 2 −∆∆CT method as described in 52 Primary patient samples. RNA was isolated from 95 patients with primary AML (FAB classification M0-M4). Patients were enrolled in and experimental protocols were approved by HOVON/SAKK (protocols −04, −04A, −29, and −42; available at www.hovon.nl) between 1987 and 2006 [55][56][57][58] . All patients provided written informed consent in accordance with the Declaration of Helsinki and all methods were performed in accordance with the relevant guidelines and regulations. After informed consent was given, bone marrow aspirates or peripheral blood samples were taken at diagnosis. Patient data are summarized in Supplementary Table 1 Long-lived protein degradation assay. NB4 cells were seeded at a density of 0.1 × 10 6 /ml and treated with vehicle, 1 µM ATRA (Sigma-Aldrich, Buchs, Switzerland) or 1 µM acitretin (Sigma-Aldrich, Buchs, Switzerland) for two days before the addition of 0.2µCi of 14 C-Valin/ml (L-(U-14-C)Valine, Code CFB.75, Amersham). Cells were incubated for another two days before the long-lived protein degradation assays were performed. Cells were washed and incubated for 1.5 h in the presence of 10 mM non-radioactive L-Valin before the 5 h chasing phase was started. Protein precipitations were carried using trichloracetic acid (at 10%) and phosphotunctic acid (at 1%). After incubation at 4 °C for 30 minutes samples were centrifuged at 600 rcf for 15 minutes. Radioactivity in the supernatant and the pellet fractions was determined using a scintillation counter (PerkinElmer). Proteolysis was calculated as the percentage of radioactivity in the supernatant.
Luciferase assay. The activity of miR-181b on the 3′UTR of ALFY was tested using the luciferase assay kit LightSwitch from SwitchGear Genomics (California, USA) according to manufacturer's instructions. Briefly, H1299 cells were seeded at a density of 20'000 cells per 96-well. 24-hours later, cells were transfected using the Lipofectamine2000 reagent (Life Technologies, Zug, Switzerland). 24-hours following transfection, luminescence was measured using Tecan Reader Infinite200 (Tecan, Switzerland). MicroRNA mimics or scrambled sequence were purchased from Qiagen (Hombrechtikon, Switzerland).
Co-Immunoprecipitation experiments. Protein lysates used for IP were prepared from HEK293T or NB4 cells. Cells were harvested and lysed in ice cold NP40 buffer (125 mM KAc, 25 mM Hepes at pH 7.2, 5 mM EDTA, 2.5 mM MgAc, 0.05% NP40 and 1 mM DTT) containing a protease and phosphatase inhibitor cocktail (Roche, 04906845001). The cell lysates were used for IP with anti-ALFY serum or pre-immune serum 21 at 4 °C for 10 to 12 h. After addition of protein A agarose beads (Amersham Biosciences, 17-0963-03) and protein G agarose beads (Amersham Biosciences, 17-0618-01), the incubation was continued for 1 h. Immunoprecipitates were washed three times with ice-cold lysis buffer and eluted with SDS loading buffer at 95 °C for 5 min.