天津地区核酸检测重复无反应性献血者HBV感染指标分析

doi:10.3969/j.issn.1671-2587.2023.03.019

临床输血与检验 ›› 2023, Vol. 25 ›› Issue (3): 395-400.DOI: 10.3969/j.issn.1671-2587.2023.03.019

天津地区核酸检测重复无反应性献血者HBV感染指标分析

李凤园, 袁玉华, 潘彤, 谢月娜, 徐姗

300110 天津血液中心（李凤园,潘彤,谢月娜）; 天津医科大学总医院（袁玉华）; 天津市胸科医院（徐姗）

收稿日期:2023-01-17 发布日期:2023-07-10
通讯作者: 袁玉华,主任技师,博士,硕士研究生导师,主要从事病原生物学相关研究,（E-mail）yyhxxx39@sina.com。
作者简介:李凤园,主管技师,硕士,主要从事血液筛查相关研究,（E-mail）lifengyuan101@126.com。

Analysis of HBV Infection Indexes in Repeated Non-Reactive Blood Donors with Nucleic Acid Test in Tianjin Area

LI Fengyuan, YUAN Yuhua, PAN Tong, et al

Tianjin Blood Center ,Tianjin 300110

Received:2023-01-17 Published:2023-07-10

摘要/Abstract

摘要： 目的使用不同类型的NAT法对HBsAg阴性的核酸检测重复无反应性（NRR）献血者样本进行检测,同时使用ELISA法对HBV DNA阳性样本进行相关标志物检测,确认HBV DNA阳性样本的血清学感染指标的模式,保障用血安全。方法使用TMA原理的单人份核酸检测（ID-NAT）对82 278例献血者样本进行检测后,总共收集60例NRR样本血浆,采用3种NAT方法对HBV DNA进行检测：方法①采用TMA原理的NAT法进行3次HBV DNA鉴别试验;方法②使用A、B不同的PCR试剂对HBV DNA进行检测;方法③使用Q-PCR对HBV DNA进行定量检测,得到3种方法的总阳性数及比率。使用ELISA法对确认HBV DNA阳性组进行血清学标志物检测,并与未确认HBV DNA阳性组进行比较,分析两组抗体和血清学组合模式阳性率有无差异。结果 60例NRR样本,方法①检出HBV DNA阳性样本19例（31.67%,19/60）,方法②检出HBV DNA阳性样本23例（38.33%,23/60）,方法③检出HBV DNA阳性样本9例（15%,9/60）且病毒载量均较低。3种方法检测出感染HBV的NRR样本共32例（53.33%,32/60）,其中仅方法①6例（18.758%,6/32）、仅方法②10例（31.25%,10/32）、仅方法③3例（9.37%,3/32）。确认组的HBcAb和阳性率高于未确认组,高达84.38%和9.38%,两组比较具有统计学差异。确认组HBcAb（+）且HBeAb（+）比率为6.25%而未确认组无此模式,所有抗体全阴性的组合模式确认组比率6.25%低于未确认组28.57%。结论多种类型的NAT法联合检测可以提高NRR样本中HBV DNA的检出率,NRR人群中确认HBV DNA阳性献血者感染标志物HBcAb阳性率、HBcAb（+）且HBeAb（+）比率均升高,所有抗体全阴性的组合模式比率降低。

关键词: 核酸检测重复无反应性, HBV, Q-PCR, ELISA

Abstract: Objective To use different types of NAT method to detect the HBsAg negative repeated non-reactive (NRR) donor samples, and ELISA method to detect the relative markers of HBV DNA positive samples, so as to confirm the changes of serological infection indexes of HBV DNA positive samples and ensure the safety of blood use. Methods A total of 60 NRR samples were collected after the detection of 82 278 blood donor samples using the TMA ID-NAT. Three different types of NAT methods were used to detect HBV DNA.Methods① HBV DNA identification tests were performed three times.Methods② HBV DNA was detected with different PCR reagents A and B. Methods③ Q-PCR was used to quantitatively detect HBV DNA, and the total positive number and ratio of the three methods were obtained. ELISA method was used to detect relevant markers in the HBV NRR donor population infected with the virus, and OBI infection situation was obtained, and then compared with the qualified donor population to analyze whether there was any difference in the ratio of antibody and serological combination mode between the two populations. Results Among the 60 NRR samples, method ①19 cases (31.67%, 19/60) were detected positive for HBV DNA, method ②23 cases (38.33%, 23/60) were detected positive for HBV DNA, method ③ 9 cases (15%, 9/60) were detected positive for HBV DNA, with low viral load. A total of 32 cases (53.33%, 32/60) of HBV-infected NRR samples were detected by the three methods, including 19 cases (59.38%, 19/32) with the method ①, 8 cases (25%, 8/32) with the method ② and 3 cases (9.37%, 3/32) with the method ③ alone. The positive rates of HBcAb (+) and combination mode 1 were statistically different between the two groups. Conclusion Multi-type NAT combined detection can improve the detection rate of HBV DNA in NRR samples and increase the detection of markers, changes in the positive rate of HBV infection markers were identified in NRR donors with positive HBV DNA.

Key words: NAT NRR, HBV, Q-PCR, ELISA

中图分类号:

R446

李凤园, 袁玉华, 潘彤, 谢月娜, 徐姗. 天津地区核酸检测重复无反应性献血者HBV感染指标分析[J]. 临床输血与检验, 2023, 25(3): 395-400.

LI Fengyuan, YUAN Yuhua, PAN Tong, et al. Analysis of HBV Infection Indexes in Repeated Non-Reactive Blood Donors with Nucleic Acid Test in Tianjin Area[J]. JOURNAL OF CLINICAL TRANSFUSION AND LABORATORY MEDICINE, 2023, 25(3): 395-400.

参考文献

[1] STOLZ M,GOWLAND P,TINGUELY C,et al.Safe-testing algorithm for individual-donation nucleic acid testing:10 years of experience in a low-prevalence country[J].Transfus Med Hemother,2019,46(2):104-110.
[2] 尹丹,欧阳熊妍,陈雪,等.重庆地区血液筛查核酸联检与鉴别检测结果不一致标本OBI确认[J].重庆医学,2020,49(20):3376-3380.
[3] 周璐. 核酸检测重复无反应性的血液HBV残留风险[D].大连:大连医科大学,2018.
[4] 邓雪莲,李婷婷,郭笑寒,等.核酸检测非重复反应性的HBsAg阴性血液HBV感染的确认[J].中国输血杂志,2018,31(9):962-967.
[5] BAKKOUR S,DENG X T,BACCHETTI P,et al.Replicate aptima assay for quantifying residual plasma viremia in individuals on antiretroviral therapy[J].J Clin Microbiol,2020,58(12):e01400-e01420.
[6] 杨宇婷. 儿童隐匿性乙肝病毒感染风险及检测方法的研究[D].重庆:重庆医科大学,2020.
[7] 易永祥. 乙型肝炎病毒的分子流行病学研究进展[J].新发传染病电子杂志,2020,5(1):1-7.
[8] 刘忠萍. 全球乙型肝炎病毒基因型和基因亚型分布的Meta分析[D].安徽医科大学,2020.
[9] AL-QAHTANI A A,POURKARIM M R,TROVÃO N S,et al.Molecular epidemiology,phylogenetic analysis and genotype distribution of hepatitis B virus in Saudi Arabia:predominance of genotype D1[J].Infect Genet Evol,2020,77:104051.
[10] GOU H N,PAN Y,GE H W,et al.Evaluation of an individual-donation nucleic acid amplification testing algorithm for detecting hepatitis B virus infection in Chinese blood donors[J].Transfusion,2015,55(9):2272-2281.
[11] HOSHI Y,HASEGAWA T,YAMAGISHI N,et al.Optimal titer of anti-HBs in blood components derived from donors with anti-HBc[J].Transfusion,2019,59(8):2602-2611.
[12] RAIMONDO G,LOCARNINI S,POLLICINO T,et al.Update of the statements on biology and clinical impact of occult hepatitis B virus infection[J].J Hepatol,2019,71(2):397-408.
[13] 叶贤林,许晓绚,邵文,等.献血者HBsAg阴性NAT可疑结果标本乙肝感染状况的调查分析[J].中国输血杂志,2019,32(8):798-802.
[14] KANG J W,SEO J H,YOUN K W,et al.Use of supplemental anti-HBc testing of donors showing non-discriminating reactive results in multiplex nucleic acid testing[J].Vox Sang,2017,112(7):622-627.

[1]	黄敏, 李燕, 张立波, 傅强. 南京地区无偿献血人群输血传播HBV残余风险度评估研究^*[J]. 临床输血与检验, 2022, 24(4): 454-458.
[2]	刘海艇, 邓智华, 蔡丹, 孟芹, 桂嵘, 王勇军, 凌锋, 王海燕, 陈军浩, 王顺, 谢华斌, 黄丽芳, 王占科, 李志波, 程金凤, 焦巍, 唐曙明, 谢小兵, 江小工, 陈亚军, 周红霞, 骆群, 黄远帅, 周明, 吕小英. 10173例检测乙型肝炎标本的血清学与核酸结果分析^*[J]. 临床输血与检验, 2020, 22(6): 583-586.
[3]	辛菊梅. 慢性乙型肝炎及肝硬化患者HBsAg和HBV DNA定量检测的临床意义[J]. 临床输血与检验, 2020, 22(2): 203-205.
[4]	陈少彬, 何子毅, 陈庆恺, 刘泽民, 王庆, 黄素媛, 陈静文, 余霖, 车嘉琳. ECLIA常规应用于献血者血液HBsAg检测的结果分析^*[J]. 临床输血与检验, 2019, 21(4): 383-386.
[5]	姚玮, 王久香, 霍星星, 周秋梅, 黄开泉. 乙型肝炎病毒基因分型与耐药突变基因位点的检测分析^*[J]. 临床输血与检验, 2019, 21(4): 428-430.
[6]	王桂喜, 汪道法. ELISA法检测抗-HIV灰区设置的探讨[J]. 临床输血与检验, 2019, 21(2): 162-165.
[7]	王湘屏, 郭建波, 段荣, 王英. 衡阳地区无偿献血者核酸检测结果分析^*[J]. 临床输血与检验, 2018, 20(6): 563-565.
[8]	徐志华, 周军兵. 2016年盐城市献血者ELISA试验室内质控结果分析[J]. 临床输血与检验, 2018, 20(5): 545-547.
[9]	胡贵宾,郑艳梅,释艳华. 襄阳地区ELISA+NAT模式降低HBV输血残余风险的效果分析*[J]. 临床输血与检验, 2018, 20(3): 273-275.
[10]	张毓, 孙国栋, 张丽, 王学刚. 9例核酸反应性标本与对应ELISA、CLIA法检测HBV的关联分析[J]. 临床输血与检验, 2018, 20(2): 206-208.
[11]	谢丽鸯, 黃莉娜, 黃丽华. 龙岩地区无偿献血人群乙肝DNA阳性情况分析[J]. 临床输血与检验, 2018, 20(1): 33-35.
[12]	金一鸣, 方志红, 陆荣. 血液筛查中1例低浓度HIV窗口期标本的检测[J]. 临床输血与检验, 2018, 20(1): 42-44.
[13]	邹宵萌. ELISA检测抗-HCV灰区、弱反应标本与FQ-PCR检测结果对比分析[J]. 临床输血与检验, 2017, 19(5): 505-507.
[14]	黄慧, 陈秀兰, 吴洁, 潘安杰, 马怡, 陈丽, 潘洁. 皖南地区血液集中化检测应用分析[J]. 临床输血与检验, 2017, 19(3): 291-294.
[15]	林诗雅, 王淏, 李仲平, 梁浩坚, 谢君谋, 肖韶英, 郑优荣. 2015年广州地区无偿献血者核酸和ELISA检测结果分析[J]. 临床输血与检验, 2017, 19(2): 137-141.

天津地区核酸检测重复无反应性献血者HBV感染指标分析

Analysis of HBV Infection Indexes in Repeated Non-Reactive Blood Donors with Nucleic Acid Test in Tianjin Area

RichHTML

PDF

可视化

摘要/Abstract

引用本文

使用本文

参考文献

相关文章 15

编辑推荐

Metrics

本文评价

关于本刊

作者中心

在线期刊

访问统计

联系我们