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本文引用的文献

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Very late antigen 4-dependent adhesion and costimulation of resting human T cells by the bacterial beta 1 integrin ligand invasin.细菌β1整合素配体侵袭素对静息人T细胞的极晚期抗原4依赖性黏附及共刺激作用。
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整联蛋白VLA-4的α4亚基中假定的二价阳离子位点的突变:对与CS1/纤连蛋白、血管细胞黏附分子-1和侵袭素黏附的不同影响。

Mutation of putative divalent cation sites in the alpha 4 subunit of the integrin VLA-4: distinct effects on adhesion to CS1/fibronectin, VCAM-1, and invasin.

作者信息

Masumoto A, Hemler M E

机构信息

Dana-Farber Cancer Institute and Harvard Medical School, Boston, Massachusetts 02115.

出版信息

J Cell Biol. 1993 Oct;123(1):245-53. doi: 10.1083/jcb.123.1.245.

DOI:10.1083/jcb.123.1.245
PMID:7691827
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2119803/
Abstract

To investigate the functional significance of putative integrin divalent cation binding sites, several mutated alpha 4 subunit cDNAs were constructed. Mutants contained the conservative substitution of Glu for Asp or Asn at the third position in each of three putative divalent cation sites. Transfection of wild-type or mutated alpha 4 into K562 cells yielded comparable expression levels and immunoprecipitation profiles. However, for all three alpha 4 mutants, adhesion to CS1/fibronectin was greatly diminished in either the presence or absence of the stimulatory anti-beta 1 mAb TS2/16. Constitutive adhesion to vascular cell adhesion molecule (VCAM) 1 was also diminished but, unlike CS1 adhesion, was restored upon TS2/16 stimulation. In contrast, adhesion to the bacterial protein invasin was minimally affected by any of the three mutations. For each of the mutants, the order of preference for divalent cations was unchanged compared to wild-type alpha 4, on CS1/fibronectin (Mn2+ > Mg2+ > Ca2+), on VCAM-1 (Mn2+ > Mg2+ = Ca2+) and on invasin (Mg2+ = Ca2+). However for the three mutants, the efficiency of divalent cation utilization was decreased. On VCAM-1, 68-108 microM Mn2+ was required to support half-maximal adhesion for the mutants compared with 14-18 microM for wild-type alpha 4. These results indicate (a) that three different ligands for VLA-4 show widely differing sensitivities to mutations within putative divalent cation sites, and (b) each of the three putative divalent cation sites in alpha 4 have comparable functional importance with respect to both divalent cation usage and cell adhesion.

摘要

为了研究假定的整合素二价阳离子结合位点的功能意义,构建了几个突变的α4亚基cDNA。突变体在三个假定的二价阳离子位点中的每一个的第三位含有将Glu保守替换为Asp或Asn。将野生型或突变型α4转染到K562细胞中产生了相当的表达水平和免疫沉淀谱。然而,对于所有三个α4突变体,无论是否存在刺激性抗β1单克隆抗体TS2/16,其对CS1/纤连蛋白的粘附都大大减少。对血管细胞粘附分子(VCAM)1的组成性粘附也减少了,但与CS1粘附不同,在TS2/16刺激后恢复。相比之下,对细菌蛋白侵袭素的粘附受这三个突变中的任何一个的影响最小。对于每个突变体,与野生型α4相比,在CS1/纤连蛋白上(Mn2+>Mg2+>Ca2+)、在VCAM-1上(Mn2+>Mg2+=Ca2+)和在侵袭素上(Mg2+=Ca2+),二价阳离子的优先顺序没有改变。然而,对于这三个突变体,二价阳离子的利用效率降低了。在VCAM-1上,突变体需要68-108μM的Mn2+来支持半最大粘附,而野生型α4则需要14-18μM。这些结果表明:(a)VLA-4的三种不同配体对假定的二价阳离子位点内的突变表现出广泛不同的敏感性;(b)α4中的三个假定的二价阳离子位点在二价阳离子使用和细胞粘附上都具有相当的功能重要性。