Sample Collection

Figure 1

Figure 1. Locations of sampling areas and of different hemagglutinin (HA) clades in study of avian influenza A(H5N1) viruses circulating in Indonesia, 2015–2016. A) West Java Province; B) location of province in Indonesia...

During April 2015–October 2016, district animal health officers of the West Java Animal Health Authority collected samples from birds in 6 districts of West Java Province: Subang, Indramayu, Tasikmalaya, Purwakarta, Sukabumi, and Bandung (Figure 1). The districts were chosen on the basis of the history and recurrence of HPAI outbreaks. In addition, these districts have multiple sectors of poultry farms using various production systems and a high density of poultry farms that have >50 birds/farm (4,16).

The samples were collected after detection of clinical signs in or increased mortality of birds. The criteria for increased mortality was set at >5% of the population in birds vaccinated against H5N1 and 10% in those unvaccinated for 2 consecutive days. When the criteria were met, oropharyngeal and cloacal samples were collected from 5 sick birds and pooled into viral transport medium containing brain–heart infusion broth and antimicrobial drugs according to European Union instructions (http://extwprlegs1.fao.org/docs/pdf/eur65757.pdf). The specimens were kept chilled and shipped by overnight courier to the 2 collaborating veterinary laboratories, Disease Investigation Center (DIC) Subang and West Java Animal Health Laboratory Cikole.

Sample Screening

We tested the collected samples in veterinary laboratories using a national protocol for influenza A screening developed from a real-time reverse transcription PCR (RT-PCR) targeting the matrix gene. Specimens with a cycle threshold value <30 were inactivated using binding buffer of High Pure Viral RNA kit (Roche Applied Science, http://www.roche.com), and transported to the Eijkman Institute for Molecular Biology in Jakarta for Sanger sequencing. Two additional HPAI H5N1–positive samples, collected in 2016 and obtained from the Animal Health Laboratory (AHL) Cikole of West Java, were also inactivated and included in this study for Sanger sequencing.

Sequencing

At the Eijkman Institute, we rescreened the specimens and extracted RNA in accordance with the protocol of the manufacturer and synthesized cDNA by Invitrogen Super Script III First-Strand Synthesis SuperMix (Thermo Fisher Scientific, http://www.thermofisher.com) with Uni12 primer (17). On specimens that tested positive in this PCR, we performed additional PCRs to amplify other gene segments present in the samples. We performed amplification of the full genomes of HPAI H5N1 viruses using a 2-step RT-PCR TaKaRa Z-Taq DNA Polymerase (Takara Bio, http://www.takarabio.com) or Toyobo KOD FX Neo (Toyobo, http://www.toyobo-global.com) if the genomes were not successfully amplified using the Takara product.

The primers used were primarily designed by Wageningen Bioveterinary Research. We obtained additional primer sequences from the Australian Animal Health Laboratory and from scientific literature (17,18) and applied them to unsuccessfully sequenced gene fragments that could not be amplified by standard primers. We purified the amplified PCR products with Roche High Pure PCR Product Purification Kit (Roche) or Zymoclean Gel DNA Recovery Kit (Zymo Research, https://www.zymoresearch.com) for PCR products for which gel separation was necessary, and subsequently sequenced them using a BigDye Terminator v3.1 Cycle Sequencing Kit in an ABI 3130 Genetic Analyzer (both from Thermo Fisher).

Genetic and Phylogenetic Analysis

Figure 2

Figure 2. Number of samples in study of avian influenza A(H5N1) viruses circulating in Indonesia, 2015–2016, by district (A), time (B), poultry type (C), poultry sector (D), and farm size (E) from which...

We assembled and edited sequences with Lasergene SeqMan Pro version 12 (DNASTAR, http://www.dnastar.com) and aligned them by using MUSCLE (19). We initially determined HA clade of sequenced HPAI H5N1 viruses using the Highly Pathogenic H5N1 Clade Classification Tool of the Influenza Research Database (https://www.fludb.org) and confirmed results through further phylogenetic analysis (20). We estimated phylogenetic inference using the maximum-likelihood method with 1,000 bootstrap replicates (Figure 2; Appendix 1 Figure 1). We chose the most suitable substitution rates and pattern model based on the lowest Akaike information criterion for each alignment. Evolutionary distances were computed using average pairwise distance (APD) between and within sequence groups. Evolutionary analyses and APD were conducted in MEGA6 (21).

We aligned the sequences of HPAI H5N1 gene segments collected during this study with reference sequences from GenBank (Appendix 1 Figures 1–8) using BLAST (https://blast.ncbi.nlm.nih.gov/Blast.cgi). We included in the analysis sequences obtained from viruses detected during other recent outbreaks in Indonesia (2014–2016). These viruses had been collected via passive outbreak surveillance by the Disease Investigation Centres (DIC) in Medan, Sumatra; Wates, Central Java; and Denpasar, Bali, under the Directorate General for Livestock and Animal Health Services and the Indonesian Ministry of Agriculture (DGLAHS-MoA). Viruses were submitted by DIC Wates of DGLAHS-MoA to GenBank, and then downloaded to GISAID (https://www.gisaid.org; accession nos. EPI1009273–463) (Appendix 2 Table 1). For sequencing, we used mainly viruses from original material, as well as some isolates obtained after 1–2 passages in embryonated chicken eggs. We deduced reassortment events on the basis of deviant location of sequences in maximum-likelihood trees of different gene segments.

We used deduced HA amino acid sequences to calculate estimated antigenic distances of viruses based on 27 aa residues in HA, as described previously (22). We measured the antigenic distances with 3 HPAI H5N1 strains that are or were routinely used to vaccinate poultry in Indonesia: A/chicken/Legok/2003 (clade 2.1.1); A/chicken/West Java/PWT-WIJ/2006 (clade 2.1.3.2); and A/duck/Sukoharjo/BBVW-1428–9/2012 (clade 2.3.2.1c). We used a t-test to estimate the significance of the comparison between the 2 averages of antigenic distances.

Detection and Sequencing of HPAI Viruses

A total of 76 pooled samples were collected from various districts of West Java, Indonesia (Figure 1). We observed the highest number of outbreaks in Indramayu in February 2016. During April 2015–October 2016, a total of 56 of the samples tested positive for influenza A virus by real-time RT-PCR with a cycle threshold value <30. We obtained the complete genome from 37 oropharyngeal samples and 2 swab specimens of the 55 samples and used these sequences in the analysis. Positive samples with complete genomes were mostly collected in Indramayu (46.15%, 95% CI 30.5%–61.8%) and Subang (38.46%, 95% CI 23.2%–53.7%); the highest peak came in February 2016 (41.3%, 95% CI 25.6%–56.5%), and most positive samples came from backyard chickens (69.23%, 95% CI 54.74%–83.71%). The positive samples were primarily from sector 4 (69.23%, 95% CI 52.4%–83%), from farms with <100 birds/farm (53.85%, 95% CI 37.2%–70%) (Figure 2). Sequences comprising the whole genome were submitted to GISAID (Appendix 2 Table 1).

Phylogenetic Analysis of HPAI H5N1 Genes

Analysis of obtained hemagglutinin (HA) and neuraminidase (NA) nucleotide and deduced amino acid sequence data confirmed that viruses in our samples were HPAI H5N1 with polybasic cleavage motif (Q-R-E-R-R-R-K-R-G-L-F) and (Q-R-E-K-R-R-K-R-G-L-F). Phylogenetic analysis showed that the HA genes of the HPAI H5N1 viruses in our study samples all belong to clade 2.3.2.1c. In-depth analysis revealed that Indonesia 2015–2016 HPAI H5N1 clade 2.3.2.1c has evolved into 2 putative new subgroups, A and B. The APD between the 2 subgroups within clade 2.3.2.1c was >1.5% (3.3% ± 0.4%); the bootstrap value was >60%; and the APDs within the 2 groups within clade 2.3.2.1c were <1.5% (0.9% ± 0.1% for subgroup A and 1.9% ± 0.2% for subgroup B). One sample collected by DIC Medan in 2016 from Sumatra Island was identified as clade 2.1.3.2a (Appendix 1 Figure 1).

We observed the evolution of clade 2.3.2.1c of Indonesia 2015–2016 HPAI H5N1 viruses into putative new subgroups (A and B) for the polymerase basic 1 (PB1), polymerase (PA), nucleoprotein (NP), and neuraminidase (NA) genes, as became apparent from comparing respective phylogenetic trees of these genes (Appendix 1 Figures 2–5). The APDs of the PB1, PA, NP, and NA genes were computed, although APD for these genes has not been used yet for HPAI nomenclature. The APD between the 2 different subgroups A and B within clade 2.3.2.1c viruses was 2.3% ±0.3% for PB1, 2.4% ±0.3% for PA, 2.1% ±0.3% for NP, and 3.4% ±0.3% for NA; and the APDs within the 2 different subgroups of clade 2.3.2.1c were 0.8% ±0.1% (A) and 1.6% ±0.2% (B) for PB1, 0.7% ±0.1% (A) and 1.3% ±0.1% (B) for PA, 0.6% ±0.1% (A) and 1.1% ±0.1% (B) for NP, and 0.7% ±0.1% (A) and 1.9% ±0.2% (B) for NA.

We identified 4 different variants of PB2 in HPAI H5N1 cases from Indonesia in 2015–2016, whereas MP and NS consisted of 3 variants. One of the 4 variants in the PB2 gene of HPAI H5N1 viruses collected by DIC from poultry outbreaks in Central and East Java in 2016 was similar to PB2 of LPAI from Asia (Appendix 1 Figures 1, 7, and 8).

Detection of Possible Reassortments

Figure 3

Figure 3. Reassortment events of avian influenza A(H5N1) viruses in samples from Indonesia, 2015–2016, some of which were confirmed using maximum-likelihood analysis with parent strains clade 2.3.2.1c, 2005-11 (clade 2.1.3.2a), and Asia low...

Analysis of obtained sequence data by the maximum-likelihood method revealed the presence of multiple reassortments of HPAI H5N1 virus gene segments of different viruses circulating in Indonesia, using viruses of clade 2.3.2.1c, 2.1.3.2a, and Asia LPAI as parent strains (Figure 3). Based on the complete genome sequences of 37 positive samples, we identified the district with the most reassorted viruses as Indramayu (20.5%, CI 95% 9.3%–36.5%). The month with the largest proportion of infections was February 2016 (18%, 95% CI 7.5%–33.5%), and the type of poultry with the largest proportion of infections was backyard chickens (15.4%, 95% CI 5.9%–30.5%). We identified ≈18% (95% CI 7.5%–33.5%) of reassorted viruses in poultry sector 4; 15.4% (95% CI 5.95%–30.5%) were in farms with <100 birds/farm (Figure 3).

Antigenic Distance Based on Genetic Distance

It has been demonstrated recently that genetic distances in 27 selected amino acid residues of the HA of HPAI H5 viruses correlate with antigenic distances (22). These 27 positions correlate closely with antigenicity and are close to receptor binding sites (23,24). We observed amino acid changes in the HA of the HPAI H5N1 viruses analyzed in our study at 19/27 selected residues: N72D, D97N, Q115H, S129L, S133A, P136S/P136L, L138Q, S140N, P141S, N154D/N154S, R162K, S163G/S163N/S163T, D183N, E184G, A185G, T188I, K189R/K189M, R212K, M226I (Appendix 2 Table 4).

Results show that the estimated average antigenic distance of HPAI H5N1 viruses from subgroup A was slightly smaller than from subgroup B to the most recent seed virus vaccine, A/duck/Sukoharjo/BBVW-1428-9/2012. Not surprisingly, these average antigenic distances were lower than to older seed vaccine strains of different clades (A/chicken/Legok/2003, A/chicken/West clade 2.1, and Java/PWT-WIJ/2006 clade 2.1.3.2). In all cases, the distance difference between subgroup A or B and the 3 seed vaccine strains was significant (p<0.05) (Appendix 2 Tables 4, 5).