首页> 美国卫生研究院文献>Journal of Clinical Microbiology >General primer polymerase chain reaction in combination with sequence analysis for identification of potentially novel human papillomavirus genotypes in cervical lesions.
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General primer polymerase chain reaction in combination with sequence analysis for identification of potentially novel human papillomavirus genotypes in cervical lesions.

机译:通用引物聚合酶链反应与序列分析相结合可鉴定宫颈病变中潜在的新型人乳头瘤病毒基因型。

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摘要

We recently described the detection of potentially novel human papillomaviruses (HPV) genotypes (HPV types X [HPV X]) in cervical smears (A. J. C. van den Brule, C. J. L. M. Meijer, V. Bakels, P. Kenemans, and J. M. M. Walboomers, J. Clin. Microbiol. 28:2739-2743, 1990) by using the general primer-mediated polymerase chain reaction method (GP-PCR). In this study, the HPV specificities of GP-PCR products were determined by sequence analyses. M13 bacteriophage clones of PCR products derived from cloned unsequenced HPV genotypes 13, 32, 35, 43, 44, 45, 51, and 56 were subjected to dideoxy sequencing. Analyses of the putative amino acid sequences of these HPV types in addition to published HPV sequence data revealed stretches of highly conserved amino acid residues present in all HPV types, resulting in an HPV amino acid consensus sequence. Subsequently, HPV X-specific PCR products found in premalignant cervical lesions (n = 3), carcinomas in situ (n = 6), and invasive cancer (n = 6) were analyzed for their nucleotide sequences. Comparison of these sequences with published HPV nucleotide sequences and data obtained in this study revealed three HPV type 35, two HPV type 45, one HPV type 51, two HPV type 56, and six unique HPV X sequences, of which three types were present in four cases of carcinomas (in situ). The nucleotide sequences determined appeared to be unique after a data bank search. Furthermore, the sequences of all HPV X isolates matched the HPV amino acid consensus sequence, thus confirming HPV specificity. This study illustrates the power of GP-PCR in combination with sequence analysis to determine HPV specificity and genotyping of PCR products derived from sequenced as well as unsequenced HPVs, including novel, not yet identified HPV types.
机译:我们最近描述了在宫颈涂片(AJC van den Brule,CJLM Meijer,V。Bakels,P。Kenemans和JMM Walboomers,J。Clin)中检测潜在的新型人类乳头瘤病毒(HPV)基因型(HPV X型[HPV X])。 Microbiol.28:2739-2743,1990)通过使用一般的引物介导的聚合酶链反应方法(GP-PCR)。在这项研究中,GP-PCR产物的HPV特异性通过序列分析确定。对来源于克隆的未测序HPV基因型13、32、35、43、44、45、51和56的PCR产物的M13噬菌体克隆进行双脱氧测序。除已公布的HPV序列数据外,对这些HPV类型的推定氨基酸序列的分析还揭示了在所有HPV类型中均存在的高度保守的氨基酸残基片段,从而形成了HPV氨基酸共有序列。随后,分析了在癌前宫颈病变(n = 3),原位癌(n = 6)和浸润性癌(n = 6)中发现的HPV X特异性PCR产物的核苷酸序列。将这些序列与已发表的HPV核苷酸序列进行比较,以及在本研究中获得的数据显示,三种HPV 35型,两种HPV 45型,一种HPV 51型,两种HPV 56型和六种独特的HPV X序列,其中三种类型存在于四例癌(原位)。在数据库搜索后,确定的核苷酸序列似乎是唯一的。此外,所有HPV X分离株的序列均与HPV氨基酸共有序列匹配,从而证实了HPV特异性。这项研究说明了GP-PCR与序列分析相结合的功能,可以确定HPV特异性和从测序的和未测序的HPV(包括新的,尚未鉴定的HPV类型)衍生的PCR产物的基因型。

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