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长期存活的非进展性1型人类免疫缺陷病毒感染者中缺陷型nef等位基因的高频率。

High frequency of defective nef alleles in a long-term survivor with nonprogressive human immunodeficiency virus type 1 infection.

作者信息

Mariani R, Kirchhoff F, Greenough T C, Sullivan J L, Desrosiers R C, Skowronski J

机构信息

Cold Spring Harbor Laboratory, New York 11724, USA.

出版信息

J Virol. 1996 Nov;70(11):7752-64. doi: 10.1128/JVI.70.11.7752-7764.1996.

Abstract

A large number of nef alleles were obtained from peripheral blood mononuclear cells (PBMC) of four long-term nonprogressing survivors of human immunodeficiency virus type 1 (HIV-1) infection and from five individuals with progressive HIV-1 infection. These primary nef alleles were characterized by DNA sequence analysis and for their ability to downregulate CD4 surface expression. Intact nef open reading frames that directed the expression of Nef protein were recovered from all of the individuals. Most of the Nef proteins derived from three of four individuals with nonprogressive infection and from all five individuals with progressive infection were functional as judged by their ability to induce a decrease in surface CD4 expression. In contrast, one individual with nonprogressive HIV-1 infection yielded an unusually high frequency of disrupted nef open reading frames and Nef proteins defective for CD4 downregulation. Approximately 70% of the nef clones obtained from the PBMC of this individual at eight time points over a 12-year period were disrupted or defective for CD4 downregulation. While functional Nef proteins were demonstrated early in the course of infection (1983), functional nef alleles have surprisingly not come to predominate over time in PBMC DNA in this individual.

摘要

从4名人类免疫缺陷病毒1型(HIV-1)感染的长期无进展存活者的外周血单个核细胞(PBMC)以及5名进行性HIV-1感染个体中获得了大量nef等位基因。通过DNA序列分析及其下调CD4表面表达的能力对这些原始nef等位基因进行了表征。从所有个体中都回收了完整的指导Nef蛋白表达的nef开放阅读框。根据其诱导表面CD4表达降低的能力判断,来自4名无进展感染个体中的3名以及所有5名进行性感染个体的大多数Nef蛋白都具有功能。相比之下,一名无进展HIV-1感染个体产生的nef开放阅读框中断和CD4下调缺陷的Nef蛋白频率异常高。在12年期间的8个时间点,从该个体的PBMC中获得的nef克隆中约70%在CD4下调方面存在中断或缺陷。虽然在感染过程早期(1983年)就证明了功能性Nef蛋白的存在,但令人惊讶的是,随着时间的推移,功能性nef等位基因在该个体的PBMC DNA中并未占主导地位。

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