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使用 U87.CD4 细胞系生成代表血浆变异体的 HIV-1 原发性分离物。

Generation of HIV-1 primary isolates representative of plasma variants using the U87.CD4 cell line.

机构信息

Laboratory of Experimental Virology, Department of Medical Microbiology, Center of Infection and Immunity Amsterdam (CINIMA), Academic Medical Center of the University of Amsterdam, The Netherlands.

出版信息

J Virol Methods. 2010 Nov;169(2):341-50. doi: 10.1016/j.jviromet.2010.08.001. Epub 2010 Aug 10.

Abstract

In order to obtain HIV-1 primary isolates in settings with limited access to donor PBMCs, a culture method was developed where patient PBMCs infected with HIV-1 were cultured together with U87.CD4 cells. Using this non-laborious method, it is possible to harvest virus solely on the basis of syncytia formation and circumventing monitoring of viral replication by CA-p24 ELISA. Primary isolates from 23 out of 33 patients (70%) were isolated successfully. From PCR amplification and sequencing of the V1V5 region of the viral gp120 envelope gene, primary isolates were compared with variants obtained from plasma and PBMCs of 13 patients. The primary isolates of seven patients (54%) resembled closely the plasma viral quasispecies, whereas different variants were isolated from the other patients (46%). Three patients harboured a dual infection, while this remained unnoticed from sequencing the plasma or PBMC compartment. The primary isolates were highly infectious for TZM-bl cells and could infect CD4-enriched lymphocytes. This study demonstrates that it is possible to grow viral isolates using a non-laborious and simple method. These isolates may be used in the field for studies on antiretroviral therapy or for vaccine trials.

摘要

为了在供体 PBMC 难以获得的情况下获得 HIV-1 原始分离物,开发了一种培养方法,即在 U87.CD4 细胞中培养感染 HIV-1 的患者 PBMC。使用这种不费力的方法,可以仅根据合胞体形成来收获病毒,并避免通过 CA-p24 ELISA 监测病毒复制。从 33 名患者中的 23 名(70%)成功分离出了原始分离物。通过对病毒 gp120 包膜基因的 V1V5 区进行 PCR 扩增和测序,将原始分离物与从 13 名患者的血浆和 PBMC 中获得的变异体进行了比较。7 名患者(54%)的原始分离物与血浆病毒准种非常相似,而其他患者(46%)则分离出不同的变异体。有 3 名患者存在双重感染,但从对血浆或 PBMC 区进行测序中未发现这种情况。原始分离物对 TZM-bl 细胞具有高度感染性,并能感染 CD4 富集的淋巴细胞。这项研究表明,使用不费力且简单的方法可以生长病毒分离物。这些分离物可用于研究抗逆转录病毒治疗或疫苗试验。

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