Mognetti B, Moussa M, Croitoru J, Menu E, Dormont D, Roques P, Chaouat G
Laboratoire de Biologie de la Relation Materno-foetale, Inserm U131, Hôpital A. Béclère, Clamart, France.
Clin Exp Immunol. 2000 Mar;119(3):486-92. doi: 10.1046/j.1365-2249.2000.01149.x.
We examined CD4 and major HIV-1 co-receptor expression by trophoblast cells (TC) from early placentas, and the permissiveness of TC for infection by several natural HIV-1 isolates in vitro. Ten early placentas (4-6 weeks of gestation) from HIV- women were obtained after elective abortion. CD4 and HIV-1 co-receptor expression by TC was examined in terms of both mRNA and protein. The same TC were then challenged with three clinical HIV isolates of known phenotype, two originating from mothers who transmitted the virus to their child and one from a vertically infected newborn. TC infection was detected by polymerase chain reaction. CD4 expression was detected in five of the 10 placentas, while membrane protein expression of CCR3, CXCR4 and CCR5 was detected in every case, despite quantitative differences among individuals. Bonzo, GPR1 and ChemR23 mRNAs were detected in all TC preparations. TC from seven out of eight placentas were permissive to HIV entry, but no productive viral replication was detected (reverse transcriptase activity in culture supernatants). Interestingly, the addition of chemokine(s) or a CD4-blocking antibody to the cultures failed to inhibit TC virus entry. These data point to marked interindividual variability in HIV co-receptor expression by trophoblast cells and show that TC from early placentas can be infected in vitro by clinical HIV-1 isolates. They also suggest that viral entry in vitro might occur through a mechanism independent of both CD4 and chemokine receptors.
我们检测了早期胎盘滋养层细胞(TC)中CD4和主要HIV-1共受体的表达,以及TC在体外对几种天然HIV-1分离株感染的易感性。从HIV阴性女性中获取10份早期胎盘(妊娠4 - 6周),这些胎盘是在选择性流产后获得的。从mRNA和蛋白质水平检测TC中CD4和HIV-1共受体的表达。然后用三种已知表型的临床HIV分离株对相同的TC进行攻击,其中两种分离株来自将病毒传播给孩子的母亲,一种来自垂直感染的新生儿。通过聚合酶链反应检测TC感染情况。在10份胎盘中有5份检测到CD4表达,而CCR3、CXCR4和CCR5的膜蛋白表达在每种情况下均被检测到,尽管个体之间存在定量差异。在所有TC制剂中均检测到Bonzo、GPR1和ChemR23 mRNA。8份胎盘中有7份的TC允许HIV进入,但未检测到有活性的病毒复制(培养上清液中的逆转录酶活性)。有趣的是,向培养物中添加趋化因子或CD4阻断抗体未能抑制TC病毒进入。这些数据表明滋养层细胞中HIV共受体表达存在明显的个体差异,并表明早期胎盘的TC在体外可被临床HIV-1分离株感染。它们还表明体外病毒进入可能通过一种独立于CD4和趋化因子受体的机制发生。