Mann D A, Frankel A D
Whitehead Institute for Biomedical Research, Cambridge, MA 02142.
EMBO J. 1991 Jul;10(7):1733-9. doi: 10.1002/j.1460-2075.1991.tb07697.x.
The human immunodeficiency virus-1 (HIV-1) Tat protein has previously been shown to transactivate the HIV-1-LTR when added exogenously to HeLa, H9 lymphocytic and U937 promonocytic cells growing in culture. Here we show that Tat enters these cells by adsorptive endocytosis. Tat appears to bind non-specifically to the cell surface, with greater than 10(7) sites per cell. A specific receptor was not detected by protein crosslinking experiments, and uptake was not affected by treating cells with trypsin, heparinase or neuraminidase. Uptake and transactivation could be inhibited by incubation with heparin, dextran sulfate, an anti-Tat monoclonal antibody, or by incubation at 4 degrees C. In contrast, transactivation by Tat was markedly stimulated by the addition of basic peptides, such as Tat 38-58 or protamine. Fluorescence experiments with rhodamine-conjugated Tat show punctate staining on the cell surface and then localization to the cytoplasm and nucleus. The lack of a specific receptor makes it unclear whether Tat uptake is biologically important in HIV infection, however, the efficiency of uptake raises the possibility that Tat may be useful for delivery of protein molecules into cells.
先前已表明,将人类免疫缺陷病毒1型(HIV-1)Tat蛋白外源添加到培养的HeLa细胞、H9淋巴细胞和U937原单核细胞中时,它可反式激活HIV-1长末端重复序列(HIV-1-LTR)。在此我们表明,Tat通过吸附性胞吞作用进入这些细胞。Tat似乎非特异性地结合到细胞表面,每个细胞有超过10^7个位点。蛋白质交联实验未检测到特异性受体,用胰蛋白酶、肝素酶或神经氨酸酶处理细胞对摄取没有影响。与肝素、硫酸葡聚糖、抗Tat单克隆抗体一起孵育或在4℃孵育可抑制摄取和反式激活。相反,添加碱性肽,如Tat 38-58或鱼精蛋白,可显著刺激Tat的反式激活。用罗丹明偶联的Tat进行的荧光实验显示,细胞表面有斑点状染色,然后定位到细胞质和细胞核。由于缺乏特异性受体,尚不清楚Tat摄取在HIV感染中是否具有生物学重要性,然而,摄取效率增加了Tat可能有助于将蛋白质分子递送至细胞的可能性。
