Introduction

Influenza A viruses (IAVs) cause infections in various avian and several mammalian species, including humans1. The genomes of IAVs are composed of eight negative sensed single stranded RNA segments2. Due to the segmented nature of the genome combinatorial exchanges of genome segments, so-called reassortments may occur when different IAVs replicate in the same host cell. This phenomenon significantly increases IAV genotypic variability and may also contribute to ad hoc shifts in viral phenotypes. Two glycoprotein species located in the viral membranes of IAVs, the haemagglutinin (HAs) and the neuraminidases (NAs), represent the major antigenic determinants that define the subtype of the virus2. Reassortment events that changed a combination of HA and NA glycoproteins and created a novel antigenic phenotype in an immunologically naïve human population have been the basis of pandemic, i.e., global waves of human IAV infections3. Only a subset of all known IAV subtypes infect mammalian species, whereas avian metapopulations perpetuate the full spectrum of 16 different HA and 9 NA entities4,5,6. The only exceptions are the recently described bat influenza viruses H17N10 and H18N11 that were up to now detected in bats only7,8.

The symptoms, if any, of IAV induced human disease vary from mild to severe respiratory disorders. However, rarely occurring severe systemic disorders with substantial fatality rates have been reported, as well9. In temperate climates, there is a sharply defined human influenza season, during which a total of 1 billion people are affected annually10. Influenza A-related diseases induced in susceptible livestock, particularly poultry and swine, are highly variable and may have economic implications due to animal losses, reduced production rates and/or trade restrictions. The severity of influenza infections in animals is, to some extent, related to the species, age and constitution of the host, but there are also influential viral determinants of pathogenicity. This is particularly true for highly pathogenic forms of avian influenza (AI) caused by certain lineages of the AIV subtypes H5 and H7. Avian infections with either of these subtypes, independent of their pathogenicity, are notifiable and call upon rigorous restriction and eradication measures (e.g. “stamping out”)11.

Due to the potentially far-reaching consequences of the detection of certain IAV subtypes, a rapid and reliable diagnostic subtyping assay is of paramount importance. Virus subtyping directly from original sample material would considerably reduce the time until diagnosis. Here, we describe a very broad molecular subtyping assay system based on reverse transcription quantitative PCR (RT-qPCR) in a multiwell layout that is easily prepared and runs on standard lab equipment. By using a hydrolysis probe technique (TaqMan®), one of the most powerful and widespread methodologies in diagnostic microbiology12 was applied. The format is referred to as the Riems Influenza A Typing Array, abbreviated RITA. The RITA assay is the first system that combines simple duplex TaqMan® reactions into one diagnostic tool, without the need for further equipment for detection or identification of 14 HA and 9 NA subtypes of influenza A viruses. More than 400 IAV isolates and clinical material from 63 swab samples were successfully subtyped to qualify this protocol as eminently suitable for routine procedures.

Materials and Methods

Viruses

Samples from 404 influenza viral strains representing 16 HA and 9 NA subtypes pre-typed (either serologically or by sequencing) at the National Reference Laboratory for Avian Influenza (NRL-AI, FLI) were used for analytical validation of the newly developed assays. These isolates are referred to as the “validation panel” throughout this manuscript. Tables 1 and 2 provide a condensed overview of the subtypes and species of origin, and supplemental Table S1 (available online) details the individual viral strains. Furthermore, to assess the applicability of RITA to investigate field samples containing various loads of IAV RNA, 62 swabs from wild birds (originating from wild bird monitoring) and swine (diagnostic samples from diseased swine herds) were tested. Sanger sequencing of amplicons generated from the field sample RNAs by pan-HA and pan NA RT-PCR-protocols13,14 (Henritzi et al. under review) was used to verify the RITA subtyping results.

Table 1 Condensed overview of the haemagglutinin subtype of viral isolates used to validate RITA.
Table 2 Summary of the neuraminidase subtypes of the viral isolates used to validate RITA.

Primers and probes

The pan-influenza A IAV-M1.2 assay15 was implemented in RITA as a control for the presence of IAV RNA in the sample tested and to provide quantification cycle values (Cq) for comparison to other HA- and NA-specific RT-qPCRs in the array. By in silico analyses of publicly available IAV sequences, primers and probes specific for the different HA and NA subtypes were identified. The primer and probe sets used in this study are detailed in Table 3. Oligos were synthesized by Metabion GmbH (Martinsried, Germany) and stored at −20 °C until use.

Table 3 Primers and probes used in this study.

RNA extraction

Viral RNA was extracted from supernatants of infected MDCK cell cultures or allantoic fluids of embryonated chicken eggs using the MagNA Pure LC Total Nucleic Acid Isolation Kit (Roche, Penzberg, Germany), according to the manufacturer’s instructions, on a MagNA Pure LC 2.0 system (Roche). Clinical material (swab samples) was extracted manually using the Qiagen Viral RNA kit (Qiagen, Hilden, Germany) or by the Qiagen MagAttract Kit operated on a KingFisher Biosprint96 device (Qiagen).

Individual RT-qPCRs and plate arrangement

All individual RT-qPCRs were performed on the Bio-Rad CFX 96 real-time PCR (Bio-Rad, Munich, Germany) platform in a 96-well format using the AgPath-ID One-Step kit (Applied Biosystems, Foster City, CA). Using a heterologous internal control system16, the integrity of the reagents was assured, and inhibition phenomena were excluded. The composition of a single reaction of 12.5 μl was as follows: 1 μl of RNase-free water, 6.25 μl of 2x RT-PCR buffer, 0.5 μl of RT-PCR Enzyme Mix, 0.25 μl of internal control template, 1 μl of primer-probe-mix for the internal control and 1 μl of IAV specific primer-probe-mix. Finally, 2.5 μl of RNA template was added. In its current lay-out, 32 wells (i.e., four eight-well stripes) of a 96 well PCR plate are used per RITA analysis. Thus, running three samples in parallel on one 96-well plate is possible. A typical lay-out of the 32 wells is depicted in supplemental Fig. S1, available online. During the setup of a plate, RNase-free water (0.5 μl), the IAV specific primer-probe-mix (1 μl) and the primer-probe-mix for the internal control (1 μl) were added to each individual well. At this stage of preparation, storage of the plate at −20 °C is possible, and bulk production of plates is advisable. After thawing the required amount of plates, the master mixes for each sample were prepared, which were composed of the RT-PCR buffer, the enzyme mix, the internal control RNA, residual water and the extracted viral RNA. Ten microliters of this mixture was added to each of the 32 wells of the test using a multi-channel pipette. Thus, a total of 80 μl of extracted RNA is required per sample to feed the 32 wells for a complete characterization. For PCR amplification, the following temperature profile was applied: 10 min at 45 °C (reverse transcription) and 10 min at 95 °C (inactivation of the reverse transcriptase/activation Taq polymerase), followed by 45 cycles of 15 sec at 95 °C (denaturation), 20 sec at 56 °C (annealing) and 30 sec at 72 °C (elongation). Fluorescence values (FAM, HEX) were collected during the annealing step.

In order to confirm the integrity of all of the target- and internal control-specific primer-probe-mixtures a positive control containing a mixture of RNA of all H and N subtypes targeted (panIAV-PC) is recommended. The panIAV-PC is a mixture of IAV-RNA from all IAV subtypes analysed in the array. However, based on the internal control system and the inclusion of the pan-influenza A IAV-M1.2 assay15, the application of RITA without the co-analysis of panIAV-PC is also valid. The analysis of RNase free water as a no template control (NTC) may identify cross-contamination of the master mix. Analysis of the NTC and the panIAV-PC was required after a new batch of arrays was produced, or the arrays were stored in the freezer for a prolonged period of time (more than 4 weeks) before use.

Results

RT-qPCRs and construction of a 32-well PCR array

By in silico analysis of published sequence data, primer and probes for the generic detection of HA subtypes H1 to H13 and H16 and all 9 NA subtypes were selected with the aim of detecting the broadest possible spectrum within a given subtype. To this end, various RT-qPCRs were newly developed, and their performance, analysed. In addition, published RT-qPCR subtyping protocols were evaluated, as well. Finally, the best performing assays were combined into the low density array referred to as “Riems Influenza A Typing Array” (RITA). The final makeup of RITA consisted of single assay detection of subtypes H4, H6, H8, H9, H11, H12, H13 and H16; two assays for H1, H2, H3, H5 and H10 detection; and three assays for H7 detection. NA subtyping was performed by single assays, except for the N3 subtype, which required two assays. This process resulted in the ultimate 32 well format RITA, which was evaluated using a selected set of 404 IAV isolates (detailed in supplemental Table S1). All samples were also run in the pan-influenza IAV-M1.2-assay15 included in the 32 well RITA to verify the presence of IAV RNA in general and to obtain an estimation of the viral genome load of each individual sample by generic amplification of a highly conserved region of genome segment 7 of all IAV isolates15.

Analytical sensitivity of RT-qPCRs

The analytical sensitivity of each single assay of RITA was evaluated using a dilution series of matching viral RNAs and compared with the Cq-values of the respective RNA obtained by the generic-influenza IAV-M1.2 test. The analyses showed that all subtype specific assays were similar sensitive as the generic-influenza assay. At the maximum 10-fold less viral RNA was detected, using the serotype specific assays compared to the generic pan-influenza test. In some cases, a better analytical sensitivity for the serotype specific assay was measured (data available upon request).

Analytical specificity of RITA

Analytical specificity was assessed by the determination of inclusivity and exclusivity on a validation panel of 404 different IAV isolates. The results are summarized in Table 4. As an example, “H1-subtype mix 3” detected 51 out of 54 H1 virus isolates correctly, whereas “H1 mix 27” detected 53 out of 54 H1 RNAs. Isolates that were not detected differed between the two assays: “H1 mix 3” did not detect A/mallard/Germany/R3036/2007 (H1N1), A/swine/Germany-NI/R369/2009 (H1N2) or A/swine/Germany/AR1372/2015, whereas “H1 mix 27” failed to detect A/England/1/1951 (H1N1). Therefore, with a combination of both H1 mixes, all H1 isolates represented in the validation panel were correctly identified as representatives of the H1-subtype. While “H1 mix 3” proved to be exclusively specific for H1, “H1-mix 27” showed a weak cross-reactivity with 37 H6 isolates and three isolates of the H8 subtype and therefore had a specificity of only 89.9%. However, it should be noted that there was a difference in the Cq-values (Δ Cq) between the true specific and the false positives of more than 10 units when comparing the pan IAV-M1.2 assay to the false positive signals, and 9 units when comparing the specific assay to the false positive reacting assay results.

Table 4 Reactivity of HA subtype-specific RT-qPCR assays used in RITA with the validation panel of 404 viral isolates.

Both H2-detecting assays were specific for subtype H2 and identified 18 out of 18 H2 isolates correctly, and an unspecific cross-reactivity was recorded for only one of the H5 isolates for the “IAV-H2-Mix 10” (Δ Cq > 10 generic assay, Δ Cq > 8 specific assays; Table 4). Furthermore, from a total of 40 H3 isolates of the validation panel, 35 were detected by “IAV-H3- Mix 3”, and 40 of 40 scored positive with the “IAV-H3-Mix 14” (Table 4). Additionally, all 17 H4 isolates were correctly identified by “IAV-H4-Mix 15” (Table 4). Specific detection of all H5 sequences was achieved by “IAV-H5a-Mix 1” (88/88) and also approximated by the “IAV-H5-Mix 1” assay (87/88). Subtype H6 sequences (in a total of 61 isolates) were all correctly evaluated by the “IAV-H6-Mix 8” assay (Table 4). Interestingly, for the complete identification of the H7 subtype sequences, three assays had to be implemented, providing the following coverage: “IAV-H7-CODA” detected 33 out of 35 correctly, with cross-reactivity with an H5 isolate, an H10 isolate and an H15 isolate; IAV-H7-Mix 2 detected 35 out of 35 correctly, with cross-reactions with six of the H10 isolates; “IAV-H7-Mix 2.2” detected all 35 isolates correctly. The nonspecific reactions again showed, in all cases, a Δ Cq > 10 compared to the specific reactions. Finally, the assays designed to detect the H8, H9, H11, H12, H13 and H16 subtypes reacted with the respective isolates and showed no cross-reactivity with any other subtypes. Nevertheless, both H10 assays exhibited nonspecific reactions in addition to the exact identification of all H10 subtypes: “IAV-H10-Mix 5” scored positive with 30 out of 40 H3 isolates with Cq-values that were at least three units higher than the values of the “IAV-M1.2” assay and the specific assay; “IAV-H10-Mix 9” scored positive with 30 out of 35 H7 isolates with a Δ Cq value of 5 compared to the IAV-M1.2 assay and Δ Cq value of >4 compared to the specific assay. However, with the redundancy of the two tests, all H10 isolates could be correctly identified.

The reactivity of the NA-subtype specific assays showed a 100% match to the applied isolates, with no cross-reactivity (Table 5).

Table 5 Reactivity of NA subtype-specific RT-qPCR assays used in RITA with the validation panel of 404 viral isolates.

Diagnostic performance of RITA

The evaluation of diagnostic sensitivity was conducted using RNA from swab samples of wild birds or pigs. In general, subtyping was successful for those samples that exhibited Cq-values <34 with the pan IAV M1.2 assay. Out of 45 swab samples originating from wild aquatic birds, 45 samples exhibited (at least one) HA result and 44 samples (at least one) NA results by using RITA (Table 6). In 16 samples, additional reactivity with further subtypes was evident. Eleven of these additional reactivities apparently paralleled those already known from the validation panel; thus, no mixed IV infections were assumed for these samples. In contrast, mixed influenza infection was suspected in four samples because similar Cq-values for two or more HA and NA subtypes were obtained from multiple subtype assays. Verification of subtypes identified by RITA was achieved for the majority of bird samples by Sanger sequencing technology. However, samples showing Cq-values >30 in the generic IAV M1.2 assay did not regularly yield specific amplicons, especially for the HA, that were suitable for Sanger sequencing. The individual reaction patterns of all diagnostic samples are summarized in Table S2. Nasal swabs from swine were also used for subtype detection. For 15 out of 17 IAV positive samples, a subtype was unambiguously assignable by RITA (Table 6). One sample showed additional (cross-) reactivity, as previously seen from the validation panel. Specific subtypes identified by RITA were confirmed by subsequent Sanger sequencing (except for one sample for which no NA amplicon was obtained; Table S2). For one nasal swab sample, a mixed infection with more than one subtype was suspected (Table 6).

Table 6 Diagnostic validation of RITA results from IAV-positive avian and porcine swab samples.

Discussion

The objective of this study was to develop and validate an RT-qPCR based subtyping tool for rapid and reliable direct subtyping of influenza A viruses from original sample material of avian and mammalian hosts. The finally validated 32-well RT-qPCR array, named RITA, allows the differentiation of 14 HA and 9 NA subtypes, as well as generic IAV RNA detection and an internal control system. The rare subtypes H14 and H15 were not implemented in this RITA version due to their minor relevance and to maintain an easy to manage format (e.g. using multiples of eight).

RT-qPCR-based nucleic acid detection techniques are routinely implemented throughout diagnostic laboratories, and the RITA protocol is easily established in such laboratories. The single tube duplex assay structure of RITA provides very high sensitivity for the individual assay, as well as a very good handling versatility, because all 32 wells can be pipetted using a multiwell pipette and a single master mix per sample. This format also offers complete flexibility to modify existing or implement new assays targeting specific clades, HA cleavage sites (pathotyping for H5 and H7 subtypes;)17, new geographical variants or assays for the identification of relevant pathogens of differential diagnostic importance. In the light of this flexibility, RITA can easily be adapted to the effects of evolutionary drift that may lead to IAV variants not only escaping vaccine-induced immunity but also routine diagnostics18. The current plate design resembling a low density PCR array format allows analysis of three samples in parallel per 96 well plate. The plates can be prepared in advance and stored at −20 °C. A storage time of nine months did not lead to a loss of sensitivity. Using plates from the freezer, the overall setup and run time of RITA was less than three hours.

Recently, Elizalde and colleagues described a molecular subtyping approach for HA subtyping of IAV19, and the use of locked nucleic acids (LNA) within the probe sequence in this method rendered the RT-qPCR assays highly subtype-specific19. LNA probes are specific to such an extent that single nucleotide polymorphism (SNP) genotyping is possible20. However, with this implement, mismatches within the LNA probe binding region are less well tolerated, and the likelihood of false negative reactions increases. In addition, LNA-containing probes are more expensive than Taqman® or minor groove binding (MGB®) probes. Using SYBR green as a non-specific detection tool, Tsukamoto and colleagues developed another RT-qPCR-based subtyping protocol for HA and NA of IAVs21. This approach was successfully applied to identify NA subtypes from wild bird samples originating from a surveillance program22. However, SYBR green-based detection is less specific than probe-based detection technologies because the fluorescent substance binds to any double-stranded DNA molecule amplified during PCR.

With RITA, we attempted to find a perfect balance between highly sensitive broad reactivity and extreme subtype specificity with the use of Taqman®/MGB-based probes and, if necessary, multiple tests per subtype. Certain performance traits of single RT-qPCRs implemented in RITA were already demonstrated in citations15,16,23,24,25,26; in addition, some newly designed assays were compared with published protocols27, produced superior results, and, hence, were included in the RITA format. However, due to the wide-stretched spectrum of the virus panel used to validate RITA, comprising more than 400 isolates, comparative analysis of every newly designed assay against published Taqman assays was not feasible. The current version of RITA is certainly aimed at a best fit to Eurasian IAVs. Yet, the flexible basis of the array system allows the adaptation/inclusion/substitution of single RT-qPCRs to create RITA formats that serve specific needs e.g. according to geography (Eurasian versus American genotypes) or epidemiology (outbreak-adapted assays) or differential diagnostics.

RITA was validated using 404 influenza A virus isolates from both avian and mammalian hosts, and unequivocal subtype identification was completely successful on virus isolates. The need to design primers and probes that guaranteed the broadest within-subtype reactivity and the inherent prerequisite of RITA to apply the same cycling conditions to all 32 assays implemented produced few trade-off effects with respect to specificity for some of the assays. Slight tendencies for the co-amplification of non-targeted HA subtypes were observed for some of the selected RT-qPCRs. However, these false amplicons were usually detected with a much lower sensitivity and thus could easily be identified as false-positives when comparing the true positive subtype-specific reactions to the Cq-values obtained in the pan IAV M1.2 assay. Nevertheless, this propensity of the RITA assays reduces only the reliability to detect minor virus species (particularly H1, H10) in mixed IAV infections. The necessity of discerning co-amplification from mixed infection became apparent when examining clinical material from swine and avian species. The mixed infection with subtypes H1 and N1 and N2 detected in one porcine nasal swab demonstrated the extraordinary capacity of RITA to identify mixed infections in one sample. Sample materials originating from aquatic wild birds also gave evidence of mixed infections by diverse influenza A virus subtypes when examined by RITA (Table 6). Mixed infections are a precondition of genome reassortment28, but discerning mixed infections by standard Sanger sequencing technologies is seriously hampered29. The current RITA protocol in principal allows the identification of mixed IAV infections, although the interpretation of data may require certain expertise and experience to distinguish true co-infections with different IAV subtypes from unintended co-amplification or sample contamination. For instance, samples that exhibit similar Cq values for two or more HA and NA subtypes likely represent true co-infections. In contrast, if a single major subtype is identified and one or more very minor subtypes are present in the sample, no clear decision is possible unless other subtyping methods (virus isolation, next-generation sequencing) produce corroborating results. Therefore, and to keep in touch with the evolution and geographic dissemination of IAVs, the single RITA assays will have to be reassessed and improved on a regular basis.

Rapid and unequivocal IAV subtype identification, ideally even in clinical samples, is the prerequisite for monitoring the evolutionary dynamics and diversity of IAVs, with special emphasis on the One Health concept. With the use of RITA, the standard diagnostic cascade recommended for the detection and characterization of IAV in avian samples is reduced to a pretesting using a pan-influenza IAV-assay to verify presence of IAV RNA in the sample and a single RITA run. Future versions of RITA are intended to hold an “avian RITA”, which includes cleavage site-specific assays for H5/H7 pathotyping and the detection of avian pathogens of differential diagnostic relevance. An envisaged “mammalian Rita” can include assays for the differential diagnosis of influenza-like illnesses, while certain “avian” subtypes can be excluded from the array.

Additional Information

How to cite this article: Hoffmann, B. et al. Riems influenza a typing array (RITA): An RT-qPCR based low density array for subtyping avian and mammalian influenza a viruses. Sci. Rep. 6, 27211; doi: 10.1038/srep27211 (2016).