Missed detections of influenza A(H1)pdm09 by real-time RT–PCR assay due to haemagglutinin sequence mutation, December 2017 to March 2018, northern Viet Nam

Missed detections of influenza A(H1)pdm09 by real-time RT–PCR assay due to haemagglutinin sequence mutation, December 2017 to March 2018, northern Viet Nam

Introduction: There are two methods of reverse transcription polymerase chain reaction (RT–PCR) that have been the common methods to detect influenza infections: conventional and real-time RT–PCR. From December 2017 to March 2018, several missed diagnoses of influenza A(H1)pdm09 using real-time RT–P...

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Main Authors: Hoang Vu Mai Phuong, Ung Thi Hong Trang, Nguyen Le Khanh Hang, Nguyen Thanh Thuy, Le Thi Thanh, Nguyen Vu Son, Nguyen Phuong Anh, Tran Thi Thu Huong, Vuong Duc Cuong, Le Quynh Mai
Format: Article
Language:English
Published: World Health Organization Regional Office for the Western Pacific 2019-03-01
Series:Western Pacific Surveillance and Response
Subjects:
A/H1pdm09
primers
probe
mismatch
sequences
Online Access:https://ojs.wpro.who.int/ojs/index.php/wpsar/article/view/654/912
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spelling doaj-96c1f77022014dae88ad68a872cd140a2021-04-02T12:05:47ZengWorld Health Organization Regional Office for the Western PacificWestern Pacific Surveillance and Response2094-73212094-73132019-03-01101323810.5365/wpsar.2018.9.3.003Missed detections of influenza A(H1)pdm09 by real-time RT–PCR assay due to haemagglutinin sequence mutation, December 2017 to March 2018, northern Viet NamHoang Vu Mai Phuong0Ung Thi Hong TrangNguyen Le Khanh HangNguyen Thanh ThuyLe Thi ThanhNguyen Vu SonNguyen Phuong AnhTran Thi Thu HuongVuong Duc CuongLe Quynh MaiNational Institute of Hygiene and Epidemiology, Hanoi, Viet NamIntroduction: There are two methods of reverse transcription polymerase chain reaction (RT–PCR) that have been the common methods to detect influenza infections: conventional and real-time RT–PCR. From December 2017 to March 2018, several missed diagnoses of influenza A(H1)pdm09 using real-time RT–PCR were reported in northern Viet Nam. This study investigated how these missed detections occurred to determine their effect on the surveillance of influenza. Methods: The haemagglutinin (HA) segments of A(H1N1)pdm09 from both real-time RT-PCR positive and negative samples were isolated and sequenced. The primer and probe sets in the HA gene were checked for mismatches, and phylogenetic analyses were performed to determine the molecular epidemiology of these viruses. Results: There were 86 positive influenza A samples; 32 were A(H1)pdm09 positive by conventional RT–PCR but were negative by real-time RT–PCR. Sequencing was conducted on 23 influenza (H1N1)pdm09 isolates that were recovered from positive samples. Eight of these were negative for A(H1)pdm09 by real-time RT–PCR. There were two different mismatches in the probe target sites of the HA gene sequences of all isolates (n = 23) with additional mismatches only at position 7 (template binding site) identified for all eight negative real-time RT–PCR isolates. The prime target sites had no mismatches. Phylogenetic analysis of the HA gene showed that both the positive and negative real-time RT–PCR isolates were grouped in clade 6B.1; however, the real-time RT–PCR negative viruses were located in a subgroup that referred to substitution I295V. Conclusion: Constant monitoring of genetic changes in the circulating influenza A(H1N1)pdm09 viruses is important for maintaining the sensitivity of molecular detection assays.https://ojs.wpro.who.int/ojs/index.php/wpsar/article/view/654/912A/H1pdm09primersprobemismatchsequences
collection DOAJ
language English
format Article
sources DOAJ
author Hoang Vu Mai Phuong
Ung Thi Hong Trang
Nguyen Le Khanh Hang
Nguyen Thanh Thuy
Le Thi Thanh
Nguyen Vu Son
Nguyen Phuong Anh
Tran Thi Thu Huong
Vuong Duc Cuong
Le Quynh Mai
spellingShingle Hoang Vu Mai Phuong
Ung Thi Hong Trang
Nguyen Le Khanh Hang
Nguyen Thanh Thuy
Le Thi Thanh
Nguyen Vu Son
Nguyen Phuong Anh
Tran Thi Thu Huong
Vuong Duc Cuong
Le Quynh Mai
Missed detections of influenza A(H1)pdm09 by real-time RT–PCR assay due to haemagglutinin sequence mutation, December 2017 to March 2018, northern Viet Nam
Western Pacific Surveillance and Response
A/H1pdm09
primers
probe
mismatch
sequences
author_facet Hoang Vu Mai Phuong
Ung Thi Hong Trang
Nguyen Le Khanh Hang
Nguyen Thanh Thuy
Le Thi Thanh
Nguyen Vu Son
Nguyen Phuong Anh
Tran Thi Thu Huong
Vuong Duc Cuong
Le Quynh Mai
author_sort Hoang Vu Mai Phuong
title Missed detections of influenza A(H1)pdm09 by real-time RT–PCR assay due to haemagglutinin sequence mutation, December 2017 to March 2018, northern Viet Nam
title_short Missed detections of influenza A(H1)pdm09 by real-time RT–PCR assay due to haemagglutinin sequence mutation, December 2017 to March 2018, northern Viet Nam
title_full Missed detections of influenza A(H1)pdm09 by real-time RT–PCR assay due to haemagglutinin sequence mutation, December 2017 to March 2018, northern Viet Nam
title_fullStr Missed detections of influenza A(H1)pdm09 by real-time RT–PCR assay due to haemagglutinin sequence mutation, December 2017 to March 2018, northern Viet Nam
title_full_unstemmed Missed detections of influenza A(H1)pdm09 by real-time RT–PCR assay due to haemagglutinin sequence mutation, December 2017 to March 2018, northern Viet Nam
title_sort missed detections of influenza a(h1)pdm09 by real-time rt–pcr assay due to haemagglutinin sequence mutation, december 2017 to march 2018, northern viet nam
publisher World Health Organization Regional Office for the Western Pacific
series Western Pacific Surveillance and Response
issn 2094-7321
2094-7313
publishDate 2019-03-01
description Introduction: There are two methods of reverse transcription polymerase chain reaction (RT–PCR) that have been the common methods to detect influenza infections: conventional and real-time RT–PCR. From December 2017 to March 2018, several missed diagnoses of influenza A(H1)pdm09 using real-time RT–PCR were reported in northern Viet Nam. This study investigated how these missed detections occurred to determine their effect on the surveillance of influenza. Methods: The haemagglutinin (HA) segments of A(H1N1)pdm09 from both real-time RT-PCR positive and negative samples were isolated and sequenced. The primer and probe sets in the HA gene were checked for mismatches, and phylogenetic analyses were performed to determine the molecular epidemiology of these viruses. Results: There were 86 positive influenza A samples; 32 were A(H1)pdm09 positive by conventional RT–PCR but were negative by real-time RT–PCR. Sequencing was conducted on 23 influenza (H1N1)pdm09 isolates that were recovered from positive samples. Eight of these were negative for A(H1)pdm09 by real-time RT–PCR. There were two different mismatches in the probe target sites of the HA gene sequences of all isolates (n = 23) with additional mismatches only at position 7 (template binding site) identified for all eight negative real-time RT–PCR isolates. The prime target sites had no mismatches. Phylogenetic analysis of the HA gene showed that both the positive and negative real-time RT–PCR isolates were grouped in clade 6B.1; however, the real-time RT–PCR negative viruses were located in a subgroup that referred to substitution I295V. Conclusion: Constant monitoring of genetic changes in the circulating influenza A(H1N1)pdm09 viruses is important for maintaining the sensitivity of molecular detection assays.
topic A/H1pdm09
primers
probe
mismatch
sequences
url https://ojs.wpro.who.int/ojs/index.php/wpsar/article/view/654/912
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