盘状盘齿钢鞘性细胞融合细胞表面糖蛋白gp138的纯化及特性研究

Kazuyoshi Suzuki, Kaichiro Yanagisawa
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引用次数: 14

摘要

Dictyostelium disideum的大囊形成是由两个相反的交配型菌株(如NC-4和HM1)之间的细胞融合引发的。当这些细胞在适当的环境条件下具有融合能力时,如前所述,NC-4和HM1菌株的细胞表面都出现了一种参与性细胞融合的特异性蛋白138 kDa。本研究对该蛋白进行了纯化和表征。138 kDa蛋白被证明是一种糖蛋白(gp138),特异性结合凝集素、WGA、Con-A或LCA,但不结合PNA、PHAE4、RCA60或RCA120。测定gp138的等电点pH值为4.5 ~ 4.9。为了再次证实之前的结果,在sds -聚丙烯酰胺凝胶电泳后,切出含有138-kDa条带的考马塞蓝染色凝胶,并获得针对该条带蛋白的抗血清。该抗血清的Fab片段完全抑制了NC-4和HM1细胞之间的性融合。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Purification and characterization of gp138, a cell surface glycoprotein involved in the sexual cell fusion of Dictyostelium discoideum

Macrocyst formation in Dictyostelium discoideum is initiated by the fusion of cells between two opposite mating-type strains, such as NC-4 and HM1. When these cells become fusion-competent under appropriate environmental conditions, a specific protein involved in sexual cell fusion, 138 kDa, appears on the cell surface of both NC-4 and HM1 strains, as reported previously. The present study was carried out to purify and characterize this protein. The 138 kDa protein was shown to be a glycoprotein (gp138) which binds specifically to lectins, WGA, Con-A or LCA, but not to PNA, PHAE4, RCA60 or RCA120. The isoelectric point of the gp138 was determined as pH 4.5-4.9. To confirm again the previous results, a Coomassie blue-stained gel containing the 138-kDa band was cut out following the SDS-polyacrylamide gel electrophoresis, and antiserum against this band protein(s) was obtained. Fab fragments of this antiserum caused the complete inhibition of sexual fusion between NC-4 and HM1 cells.

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