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菜豆同工凝集素亚基的重组

Recombinations of subunits of Phaseolus vulgaris isolectins.

作者信息

Felsted R L, Egorin M J, Leavitt R D, Bachur N R

出版信息

J Biol Chem. 1977 May 10;252(9):2967-71.

PMID:856807
Abstract

Phaseolus vulgaris phytohemagglutinin is formed in vivo by the combination of erythrocyte (E)-reactive and lymphocyte (L)-reactive subunits into five tetrameric isolectins:L4,L3E1, L2E2, L1E3, and E4. Evidence for phytohemagglutinin subunit structure is obtained by in vitro dissociation of native isolectins in 6 M guanidine HCl followed by removal of dissociating agents to allow subunit recombination. Dissociation and recombination of L4 yielded a single protein, electrophoretically indistinguishable from the native L4. Similar treatment of E4 also yielded a single protein indistinguishable from native E4. Treatment of L3E1, L2E2, L1E3, or a mixture of L4 and E4, yielded five distinct proteins electrophoretically similar to all five native phytohemagglutinin isolectins. Milligram quantities of all five recombinant isolectins were prepared either from L2E2 or a mixture of L4 and L1E3 proportioned to yield equimolar quantitives of the two subunits on dissociation. The recombinant isolectins were purified by affinity and SP-Sephadex ion exchange chromatography. Electrophoretic and chromatographic properties and the erythroagglutinating and mitogenic activities of recombinant isolectins were essentially identical with the native isolectins. The inclusion of 125I-labeled L4 in the dissociation results in a distribution of 125I-labeled L subunit among the purified recombinant isolectins proportional to their proposed subunit structures.

摘要

菜豆植物血凝素在体内由红细胞(E)反应性亚基和淋巴细胞(L)反应性亚基组合形成五种四聚体异凝集素:L4、L3E1、L2E2、L1E3和E4。通过在6M盐酸胍中对天然异凝集素进行体外解离,然后去除解离剂以允许亚基重组,获得了植物血凝素亚基结构的证据。L4的解离和重组产生了一种单一蛋白质,在电泳上与天然L4无法区分。对E4进行类似处理也产生了一种与天然E4无法区分的单一蛋白质。对L3E1、L2E2、L1E3或L4和E4的混合物进行处理,产生了五种不同的蛋白质,在电泳上与所有五种天然植物血凝素异凝集素相似。从L2E2或按解离时产生等摩尔量的两个亚基的比例混合的L4和L1E3中制备了毫克量的所有五种重组异凝集素。重组异凝集素通过亲和色谱和SP-葡聚糖凝胶离子交换色谱进行纯化。重组异凝集素的电泳和色谱性质以及红细胞凝集和促有丝分裂活性与天然异凝集素基本相同。在解离过程中加入125I标记的L4,会使125I标记的L亚基在纯化的重组异凝集素中的分布与其推测的亚基结构成比例。

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