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辛德毕斯病毒E2蛋白膜结合区域的突变体。I. 细胞表面转运与融合活性。

Mutants of the membrane-binding region of Semliki Forest virus E2 protein. I. Cell surface transport and fusogenic activity.

作者信息

Cutler D F, Garoff H

出版信息

J Cell Biol. 1986 Mar;102(3):889-901. doi: 10.1083/jcb.102.3.889.

Abstract

Three mutations of the membrane-binding region of the Semliki Forest virus (SFV) p62 polypeptide (the precursor for virion E3 and E2) have been made by oligonucleotide-directed mutagenesis of a cDNA clone encoding the SFV structural proteins. One of the mutations (A2) substitutes a Glu for an Ala in the middle of the hydrophobic stretch which spans the bilayer. A1 and A3 alter the two basic charged amino acids in the cytoplasmic domain next to the hydrophobic region. The wild-type charge cluster of Arg-Ser-Lys (+2) has been changed to Gly-Ser-Met (0;A3) or to Gly-Ser-Glu (-1;A1). The mutant p62 proteins have been analyzed both in the presence and the absence of E1, the other half of the heterodimer spike complex of SFV. The mutant proteins expressed in COS-7 cells are glycosylated and are of the expected sizes. When co-expressed with E1, all three mutants are cleaved to yield the E2 protein and transported to the surface of COS-7 cells. When expressed in the absence of E1, the mutant p62 proteins remain uncleaved but still reach the cell surface. Once at the cell surface, all three mutants, when co-expressed with E1, can promote low pH-triggered cell-cell fusion. These results show that the three mutant p62/E2 proteins are still membrane associated in a functionally unaltered way.

摘要

通过对编码塞姆利基森林病毒(SFV)结构蛋白的cDNA克隆进行寡核苷酸定向诱变,对SFV p62多肽(病毒粒子E3和E2的前体)的膜结合区域进行了三个突变。其中一个突变(A2)在跨越双层的疏水片段中间用谷氨酸替代了丙氨酸。A1和A3改变了疏水区域旁边胞质结构域中的两个带正电荷的氨基酸。精氨酸-丝氨酸-赖氨酸(+2)的野生型电荷簇已变为甘氨酸-丝氨酸-甲硫氨酸(0;A3)或甘氨酸-丝氨酸-谷氨酸(-1;A1)。在存在和不存在E1(SFV异二聚体刺突复合物的另一半)的情况下,对突变型p62蛋白进行了分析。在COS-7细胞中表达的突变蛋白被糖基化,且大小符合预期。当与E1共表达时,所有三个突变体都被切割产生E2蛋白,并转运到COS-7细胞表面。当在没有E1的情况下表达时,突变型p62蛋白未被切割,但仍能到达细胞表面。一旦到达细胞表面,当与E1共表达时,所有三个突变体都能促进低pH触发的细胞-细胞融合。这些结果表明,三种突变型p62/E2蛋白仍以功能未改变的方式与膜结合。

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