Djeneba Bocar Fofana , Tenin Aminatou Coulibaly , Mamoudou Maiga , Thuy Nguyen , Joël Gozlan , Zoumana Diarra , Amadou Koné , Yacouba Cissoko , Almoustapha Issiaka Maiga , Claudia A. Hawkins , Robert L. Murphy , Laurence Morand-Joubert , Mahamadou Diakité , Jane L. Holl , Sally M. McFall
{"title":"用于中低收入国家同时定量检测人类免疫缺陷病毒和乙型肝炎病毒的多重实时 PCR 检测法。","authors":"Djeneba Bocar Fofana , Tenin Aminatou Coulibaly , Mamoudou Maiga , Thuy Nguyen , Joël Gozlan , Zoumana Diarra , Amadou Koné , Yacouba Cissoko , Almoustapha Issiaka Maiga , Claudia A. Hawkins , Robert L. Murphy , Laurence Morand-Joubert , Mahamadou Diakité , Jane L. Holl , Sally M. McFall","doi":"10.1016/j.jviromet.2024.115026","DOIUrl":null,"url":null,"abstract":"<div><p>Due to shared routes of transmission, including sexual contact and vertical transmission, HIV-HBV co-infection is common, particularly in sub-Saharan Africa. Measurement of viral load (VL), for both HIV and HBV, plays a critical role for determining their infectious phase and monitoring response to antiviral therapy. Implementation of viral load testing in clinical settings is a significant challenge in resource-limited countries, notably because of cost and availability issues. We designed HIV and HBV primers for conserved regions of the HIV and HBV genomes that were specifically adapted to viral strains circulating in West Africa that are HIV-1 subtype CRF02AG and HBV genotype E. We first validated two monoplex qPCR assays for individual quantification and, then developed a multiplex qPCR for simultaneous quantification of both viruses. HIV RNA and HBV DNA amplification was performed in a single tube using a one-step reverse transcription-PCR reaction with primers and probes targeting both viruses. Performance characteristics such as the quantification range, sensitivity, and specificity of this multiplex qPCR assay were compared to reference qPCR tests for both HIV and HBV viral load quantification. The multiplex assay was validated using clinical samples from co- or mono-infected patients and gave comparable viral load quantification to the HIV and HBV reference test respectively. The multiplex qPCR demonstrated an overall sensitivity of 71.25 % [68.16–74.3] for HBV and 82 % [78.09–85.90] for HIV and an overall specificity of 100 % [94.95–100] for both viruses. Although the overall sensitivities of the HIV and HBV assays were lower than the commercial comparator assays, the sensitivity in the clinical decision range of >1000 copies/mL for HIV was 80 % [71.26–88.73] and >1000 IU/mL for HBV was 100 % [95.51–100] which indicates the test results can be used to guide treatment decisions. This in-house developed multiplex qPCR assay represents a useful diagnostic tool as it can be performed on affordable \"open\" real-time PCR platforms currently used for HIV or SARS-Cov-2 infection surveillance in Mali.</p></div>","PeriodicalId":17663,"journal":{"name":"Journal of virological methods","volume":"330 ","pages":"Article 115026"},"PeriodicalIF":2.2000,"publicationDate":"2024-09-02","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"https://www.sciencedirect.com/science/article/pii/S0166093424001502/pdfft?md5=64b2576d2db01c1ff58c5c33ea5545ae&pid=1-s2.0-S0166093424001502-main.pdf","citationCount":"0","resultStr":"{\"title\":\"A multiplexed real‐time PCR assay for simultaneous quantification of human immunodeficiency virus and Hepatitis B virus for low‐and‐middle‐ income countries\",\"authors\":\"Djeneba Bocar Fofana , Tenin Aminatou Coulibaly , Mamoudou Maiga , Thuy Nguyen , Joël Gozlan , Zoumana Diarra , Amadou Koné , Yacouba Cissoko , Almoustapha Issiaka Maiga , Claudia A. Hawkins , Robert L. Murphy , Laurence Morand-Joubert , Mahamadou Diakité , Jane L. Holl , Sally M. McFall\",\"doi\":\"10.1016/j.jviromet.2024.115026\",\"DOIUrl\":null,\"url\":null,\"abstract\":\"<div><p>Due to shared routes of transmission, including sexual contact and vertical transmission, HIV-HBV co-infection is common, particularly in sub-Saharan Africa. Measurement of viral load (VL), for both HIV and HBV, plays a critical role for determining their infectious phase and monitoring response to antiviral therapy. Implementation of viral load testing in clinical settings is a significant challenge in resource-limited countries, notably because of cost and availability issues. We designed HIV and HBV primers for conserved regions of the HIV and HBV genomes that were specifically adapted to viral strains circulating in West Africa that are HIV-1 subtype CRF02AG and HBV genotype E. We first validated two monoplex qPCR assays for individual quantification and, then developed a multiplex qPCR for simultaneous quantification of both viruses. HIV RNA and HBV DNA amplification was performed in a single tube using a one-step reverse transcription-PCR reaction with primers and probes targeting both viruses. Performance characteristics such as the quantification range, sensitivity, and specificity of this multiplex qPCR assay were compared to reference qPCR tests for both HIV and HBV viral load quantification. The multiplex assay was validated using clinical samples from co- or mono-infected patients and gave comparable viral load quantification to the HIV and HBV reference test respectively. The multiplex qPCR demonstrated an overall sensitivity of 71.25 % [68.16–74.3] for HBV and 82 % [78.09–85.90] for HIV and an overall specificity of 100 % [94.95–100] for both viruses. Although the overall sensitivities of the HIV and HBV assays were lower than the commercial comparator assays, the sensitivity in the clinical decision range of >1000 copies/mL for HIV was 80 % [71.26–88.73] and >1000 IU/mL for HBV was 100 % [95.51–100] which indicates the test results can be used to guide treatment decisions. This in-house developed multiplex qPCR assay represents a useful diagnostic tool as it can be performed on affordable \\\"open\\\" real-time PCR platforms currently used for HIV or SARS-Cov-2 infection surveillance in Mali.</p></div>\",\"PeriodicalId\":17663,\"journal\":{\"name\":\"Journal of virological methods\",\"volume\":\"330 \",\"pages\":\"Article 115026\"},\"PeriodicalIF\":2.2000,\"publicationDate\":\"2024-09-02\",\"publicationTypes\":\"Journal Article\",\"fieldsOfStudy\":null,\"isOpenAccess\":false,\"openAccessPdf\":\"https://www.sciencedirect.com/science/article/pii/S0166093424001502/pdfft?md5=64b2576d2db01c1ff58c5c33ea5545ae&pid=1-s2.0-S0166093424001502-main.pdf\",\"citationCount\":\"0\",\"resultStr\":null,\"platform\":\"Semanticscholar\",\"paperid\":null,\"PeriodicalName\":\"Journal of virological methods\",\"FirstCategoryId\":\"3\",\"ListUrlMain\":\"https://www.sciencedirect.com/science/article/pii/S0166093424001502\",\"RegionNum\":4,\"RegionCategory\":\"医学\",\"ArticlePicture\":[],\"TitleCN\":null,\"AbstractTextCN\":null,\"PMCID\":null,\"EPubDate\":\"\",\"PubModel\":\"\",\"JCR\":\"Q3\",\"JCRName\":\"BIOCHEMICAL RESEARCH METHODS\",\"Score\":null,\"Total\":0}","platform":"Semanticscholar","paperid":null,"PeriodicalName":"Journal of virological methods","FirstCategoryId":"3","ListUrlMain":"https://www.sciencedirect.com/science/article/pii/S0166093424001502","RegionNum":4,"RegionCategory":"医学","ArticlePicture":[],"TitleCN":null,"AbstractTextCN":null,"PMCID":null,"EPubDate":"","PubModel":"","JCR":"Q3","JCRName":"BIOCHEMICAL RESEARCH METHODS","Score":null,"Total":0}
引用次数: 0
摘要
由于共同的传播途径,包括性接触和垂直传播,HIV-HBV 合并感染很常见,尤其是在撒哈拉以南非洲地区。测量 HIV 和 HBV 的病毒载量(VL)对于确定其感染阶段和监测对抗病毒治疗的反应起着至关重要的作用。在资源有限的国家,在临床环境中实施病毒载量检测是一项重大挑战,主要是因为成本和可用性问题。我们针对 HIV 和 HBV 基因组的保守区域设计了 HIV 和 HBV 引物,这些引物专门适用于西非流行的 HIV-1 亚型 CRF02AG 和 HBV 基因型 E 病毒株。HIV RNA 和 HBV DNA 扩增在单管中进行,使用针对两种病毒的引物和探针,一步完成反转录-PCR 反应。将该多重 qPCR 检测法的性能特征(如定量范围、灵敏度和特异性)与 HIV 和 HBV 病毒载量定量参考 qPCR 检测法进行了比较。使用共同或单一感染患者的临床样本对该多重检测方法进行了验证,其病毒载量定量结果分别与 HIV 和 HBV 参考检测结果相当。多重 qPCR 对 HBV 和 HIV 的总体灵敏度分别为 71.25%[68.16-74.3] 和 82%[78.09-85.90] ,对这两种病毒的总体特异性均为 100%[94.95-100]。虽然 HIV 和 HBV 检测方法的总体灵敏度低于商业对比检测方法,但在 >1000 拷贝/毫升的临床决策范围内,HIV 的灵敏度为 80% [71.26-88.73] ,而 HBV >1000 IU/mL 的灵敏度为 100% [95.51-100],这表明检测结果可用于指导治疗决策。这种内部开发的多重 qPCR 分析是一种有用的诊断工具,因为它可以在马里目前用于 HIV 或 SARS-Cov-2 感染监测的经济实惠的 "开放式 "实时 PCR 平台上进行。
A multiplexed real‐time PCR assay for simultaneous quantification of human immunodeficiency virus and Hepatitis B virus for low‐and‐middle‐ income countries
Due to shared routes of transmission, including sexual contact and vertical transmission, HIV-HBV co-infection is common, particularly in sub-Saharan Africa. Measurement of viral load (VL), for both HIV and HBV, plays a critical role for determining their infectious phase and monitoring response to antiviral therapy. Implementation of viral load testing in clinical settings is a significant challenge in resource-limited countries, notably because of cost and availability issues. We designed HIV and HBV primers for conserved regions of the HIV and HBV genomes that were specifically adapted to viral strains circulating in West Africa that are HIV-1 subtype CRF02AG and HBV genotype E. We first validated two monoplex qPCR assays for individual quantification and, then developed a multiplex qPCR for simultaneous quantification of both viruses. HIV RNA and HBV DNA amplification was performed in a single tube using a one-step reverse transcription-PCR reaction with primers and probes targeting both viruses. Performance characteristics such as the quantification range, sensitivity, and specificity of this multiplex qPCR assay were compared to reference qPCR tests for both HIV and HBV viral load quantification. The multiplex assay was validated using clinical samples from co- or mono-infected patients and gave comparable viral load quantification to the HIV and HBV reference test respectively. The multiplex qPCR demonstrated an overall sensitivity of 71.25 % [68.16–74.3] for HBV and 82 % [78.09–85.90] for HIV and an overall specificity of 100 % [94.95–100] for both viruses. Although the overall sensitivities of the HIV and HBV assays were lower than the commercial comparator assays, the sensitivity in the clinical decision range of >1000 copies/mL for HIV was 80 % [71.26–88.73] and >1000 IU/mL for HBV was 100 % [95.51–100] which indicates the test results can be used to guide treatment decisions. This in-house developed multiplex qPCR assay represents a useful diagnostic tool as it can be performed on affordable "open" real-time PCR platforms currently used for HIV or SARS-Cov-2 infection surveillance in Mali.
期刊介绍:
The Journal of Virological Methods focuses on original, high quality research papers that describe novel and comprehensively tested methods which enhance human, animal, plant, bacterial or environmental virology and prions research and discovery.
The methods may include, but not limited to, the study of:
Viral components and morphology-
Virus isolation, propagation and development of viral vectors-
Viral pathogenesis, oncogenesis, vaccines and antivirals-
Virus replication, host-pathogen interactions and responses-
Virus transmission, prevention, control and treatment-
Viral metagenomics and virome-
Virus ecology, adaption and evolution-
Applied virology such as nanotechnology-
Viral diagnosis with novelty and comprehensive evaluation.
We seek articles, systematic reviews, meta-analyses and laboratory protocols that include comprehensive technical details with statistical confirmations that provide validations against current best practice, international standards or quality assurance programs and which advance knowledge in virology leading to improved medical, veterinary or agricultural practices and management.