Genotyping Human Papillomavirus in Women Attending Cervical Cancer Screening Clinic in Harare, Zimbabwe

Takudzwa Matuvhunye, Racheal Dube-Mandishora, N. Chin’ombe, G. Chakafana, J. Mbanga, E. Zumbika, B. Stray-Pedersen
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引用次数: 3

Abstract

Aim: To determine the prevalence of human papillomavirus genotypes in women attending a cervical cancer screening VIAC (visual inspection with acetic acid) clinic. Study Design: Cross-sectional study. Place and Duration of Study: VIAC clinic at Parirenyatwa Referral Hospital in Harare in Zimbabwe between February and April 2015. Methodology: Sexually active women were recruited and they provided their socio-demographic data and self-collected vaginal swabs. HIV status of the participants was determined. DNA was Original Research Article Matuvhunye et al.; BMRJ, 16(6): 1-9, 2016; Article no.BMRJ.28481 2 extracted from the swabs using the standard phenol-chloroform method. HPV DNA was detected using the standard consensus MY09/11-GP5+/GP6+ nested polymerase chain reaction. Amplicons were sequenced and sequences analyzed using bioinformatics tools to identify the HPV genotypes. Results: Sixty women were recruited. Their age ranged from 21-83 years, with a mean of 40.1 years. Most of the women were married and resided in the urban areas. Of the 60 participants, 50% (30/60) were HIV-positive. The prevalence of HPV genotypes in the study subjects was 56.7% (34/60). HPVs were most prevalent in women aged 30 years and below, and became less prevalent as the age increased. The predominant genotypes detected were HPV-16, -58, -52, -45, 18, -33, -51, -6, -81, -11, -70, -62, -32 and -40. Conclusion: A number of HPV genotypes were detected in half of women tested. There was no significance association between risk-factors (parity, level of education, residence, history of STI, contraceptive use and sexual debut) and HPV infection. The findings of this study showed that consensus nested PCR and DNA sequencing could be used to detect HPV genotypes in women in cervical cancer screening programs. Although this method is sensitive, it is inefficient at detecting multiple HPV infections.
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在津巴布韦哈拉雷参加子宫颈癌筛查诊所的妇女的人类乳头瘤病毒基因分型
目的:了解人乳头瘤病毒基因型在参加宫颈癌筛查VIAC(醋酸目视检查)门诊妇女中的流行情况。研究设计:横断面研究。研究地点和时间:2015年2月至4月,在津巴布韦哈拉雷Parirenyatwa转诊医院VIAC诊所。方法:招募性活跃的妇女,并提供她们的社会人口统计数据和自行收集的阴道拭子。确定参与者的艾滋病毒状况。DNA为原创研究文章Matuvhunye et al;中国生物医学工程学报,16(6):1-9,2016;文章no.BMRJ。28481 2用标准酚-氯仿法从拭子中提取。采用标准共识MY09/11-GP5+/GP6+巢式聚合酶链反应检测HPV DNA。扩增子测序和序列分析使用生物信息学工具,以确定HPV基因型。结果:招募了60名女性。年龄21 ~ 83岁,平均40.1岁。大多数妇女已婚,居住在城市地区。在60名参与者中,50%(30/60)是hiv阳性。研究对象中HPV基因型患病率为56.7%(34/60)。hpv在30岁及以下的女性中最流行,随着年龄的增长而变得不那么流行。检测到的主要基因型为HPV-16、-58、-52、-45、18、-33、-51、-6、-81、-11、-70、-62、-32和-40。结论:半数女性检测到多种HPV基因型。危险因素(胎次、教育水平、居住地、性传播感染史、使用避孕药具和初次性行为)与HPV感染之间无显著相关性。本研究结果表明,巢式PCR和DNA测序可用于检测宫颈癌筛查项目中妇女的HPV基因型。虽然这种方法是敏感的,但它在检测多种HPV感染方面效率低下。
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