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通过聚合酶链反应扩增、限制性片段长度多态性、核苷酸序列分析及系统发育算法对已知和新型人乳头瘤病毒进行鉴定与评估。

Identification and assessment of known and novel human papillomaviruses by polymerase chain reaction amplification, restriction fragment length polymorphisms, nucleotide sequence, and phylogenetic algorithms.

作者信息

Bernard H U, Chan S Y, Manos M M, Ong C K, Villa L L, Delius H, Peyton C L, Bauer H M, Wheeler C M

机构信息

Laboratory for Papillomavirus Biology, National University of Singapore.

出版信息

J Infect Dis. 1994 Nov;170(5):1077-85. doi: 10.1093/infdis/170.5.1077.

DOI:10.1093/infdis/170.5.1077
PMID:7963696
Abstract

The identification and taxonomy of papillomaviruses has become increasingly complex, as approximately 70 human papillomavirus (HPV) types have been described and novel HPV genomes continue to be identified. Methods and corresponding DNA sequence data bases were designed for the reliable identification of mucosal HPV genomes from clinical specimens. HPVs are identified by the amplification of a fragment of the L1 region by consensus primer polymerase chain reaction (PCR) and subsequent hybridization or restriction fragment length polymorphism analysis. L1 PCR fragments may be further characterized by nucleotide sequencing. Conservation of 30 (of 151) predicted amino acids identifies HPV genomic fragments, and nucleotide sequence alignments allow calculation of their phylogenetic relatedness. Sequence differences > 10% from any known HPV type suggest a novel HPV type. Phylogenetic relationships with known HPV types may permit predictions of biology. With these criteria, 10 PCR fragments were identified that would qualify as new genital HPV types after complete genomic isolation.

摘要

乳头瘤病毒的鉴定和分类已变得日益复杂,因为已描述了约70种人乳头瘤病毒(HPV)类型,并且仍不断发现新的HPV基因组。设计了方法及相应的DNA序列数据库,用于从临床标本中可靠鉴定黏膜HPV基因组。通过用共识引物聚合酶链反应(PCR)扩增L1区域的片段,随后进行杂交或限制性片段长度多态性分析来鉴定HPV。L1 PCR片段可通过核苷酸测序进一步表征。151个预测氨基酸中的30个的保守性可鉴定HPV基因组片段,核苷酸序列比对可计算它们的系统发育相关性。与任何已知HPV类型的序列差异> 10%提示为一种新的HPV类型。与已知HPV类型的系统发育关系可能有助于预测生物学特性。根据这些标准,鉴定出10个PCR片段,在完全分离基因组后将符合新的生殖器HPV类型的标准。

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