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用于检测慢病毒前病毒DNA的新型引物组的鉴定与评估

Identification and evaluation of new primer sets for the detection of lentivirus proviral DNA.

作者信息

Gelman I H, Zhang J, Hailman E, Hanafusa H, Morse S S

机构信息

Department of Microbiology, Mount Sinai Medical Center, New York, NY 10029.

出版信息

AIDS Res Hum Retroviruses. 1992 Dec;8(12):1981-9. doi: 10.1089/aid.1992.8.1981.

DOI:10.1089/aid.1992.8.1981
PMID:1337258
Abstract

We have developed sets of degenerate oligonucleotides designed to detect pol gene sequences from any member of the lentivirus subfamily when used as primers in amplification techniques such as the polymerase chain reaction (PCR). This pan-lentivirus-specific primer set (PLSPS) consists of primers, LV1, LV2, and LV3, based on conserved regions common to lentiviruses only. Our protocol is based on primary amplification with LV1 and LV2 followed by secondary amplification with a nested primer set based on the YM/VDD motif found in all reverse transcriptases (or "DDMY," in the opposite direction), and LV3, a block of lentivirus homology nested just downstream of LV1. PLSPS-PCR analysis of DNA from cells infected with HIV-1, HIV-2, SIVmac239, BIV, visna, EIAV, CAEV, OPPV, or FIV resulted in the amplification of appropriately sized products. Sequence analysis of the LV1/2 products, cloned into pBluescript (pBS), indicated that at least 20% (most often, > 80%) contained the predicted lentivirus pol sequence. Greater than 95% of the LV3/DDMY products contained the expected lentiviral sequences. Using the PLSPS, lentivirus pol sequences could typically be detected at levels of one copy in 2 x 10(6) cells after secondary amplification. No specific lentiviral PCR products were detected in DNA from uninfected human or mouse monocytes, feline or bovine leukocytes, mouse, rat or human fibroblast cell lines, chicken embryo fibroblasts, Tahr lung cells, or cell lines infected with the following retroviruses which are not lentiviruses: Rous sarcoma virus, Moloney leukemia virus or Kirsten sarcoma virus, mouse mammary tumor virus, human T-cell lymphotropic virus I, and feline leukemia virus.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

我们已经开发出了多组简并寡核苷酸,当用作聚合酶链反应(PCR)等扩增技术的引物时,可用于检测慢病毒亚科任何成员的pol基因序列。这种全慢病毒特异性引物组(PLSPS)由引物LV1、LV2和LV3组成,它们仅基于慢病毒共有的保守区域。我们的方案基于先用LV1和LV2进行一次扩增,然后用基于所有逆转录酶中发现的YM/VDD基序(或相反方向的“DDMY”)的巢式引物组以及LV3进行二次扩增,LV3是一段位于LV1下游的慢病毒同源序列块。对感染HIV-1、HIV-2、SIVmac239、BIV、维斯纳病毒、马传染性贫血病毒、山羊关节炎脑炎病毒、OPP病毒或猫免疫缺陷病毒的细胞DNA进行PLSPS-PCR分析,得到了大小合适的扩增产物。对克隆到pBluescript(pBS)中的LV1/2产物进行序列分析表明,至少20%(大多数情况下,>80%)含有预测的慢病毒pol序列。超过95%的LV3/DDMY产物含有预期的慢病毒序列。使用PLSPS,二次扩增后通常可以在2×10(6)个细胞中检测到一个拷贝水平的慢病毒pol序列。在未感染的人或小鼠单核细胞、猫或牛白细胞、小鼠、大鼠或人成纤维细胞系、鸡胚成纤维细胞、塔尔羊肺细胞或感染以下非慢病毒逆转录病毒的细胞系(劳氏肉瘤病毒、莫洛尼白血病病毒或克里斯滕肉瘤病毒、小鼠乳腺肿瘤病毒、人类嗜T细胞病毒I和猫白血病病毒)的DNA中未检测到特异性慢病毒PCR产物。(摘要截断于250字)

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