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2
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本文引用的文献

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Monoclonal antibodies to mouse MHC antigens. II. Antibodies to the H-2Ld antigen, the products of a third polymorphic locus of the mouse major histocompatibility complex.针对小鼠MHC抗原的单克隆抗体。II. 针对H-2Ld抗原的抗体,小鼠主要组织相容性复合体第三个多态性位点的产物
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Clonal analysis of B- and T-cell responses to Ia antigens. I. Topology of epitope regions on I-Ak and I-Ek molecules analyzed with 35 monoclonal alloantibodies.B细胞和T细胞对Ia抗原反应的克隆分析。I. 用35种单克隆同种异体抗体分析I-Ak和I-Ek分子上表位区域的拓扑结构。
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Matrix control of protein diffusion in biological membranes.生物膜中蛋白质扩散的基质控制
Proc Natl Acad Sci U S A. 1981 Jun;78(6):3576-80. doi: 10.1073/pnas.78.6.3576.
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International workshop on the application of fluorescence photobleaching techniques to problems in cell biology.荧光漂白技术在细胞生物学问题中的应用国际研讨会
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Lateral diffusion of H-2 antigens on mouse fibroblasts.H-2抗原在小鼠成纤维细胞上的侧向扩散。
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Lateral diffusion of wild-type and mutant Ld antigens in L cells.野生型和突变型利什曼原虫(Ld)抗原在L细胞中的侧向扩散。
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Transformation of mammalian cells to antibiotic resistance with a bacterial gene under control of the SV40 early region promoter.利用处于SV40早期区域启动子控制下的细菌基因将哺乳动物细胞转化为抗生素抗性细胞。
J Mol Appl Genet. 1982;1(4):327-41.
8
The interaction of lymphocyte membrane proteins with the lymphocyte cytoskeletal matrix.淋巴细胞膜蛋白与淋巴细胞细胞骨架基质的相互作用。
J Immunol. 1984 Nov;133(5):2767-72.
9
Clonal variation in cell surface display of an H-2 protein lacking a cytoplasmic tail.缺乏细胞质尾巴的H-2蛋白在细胞表面展示中的克隆变异。
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10
Transmembrane signaling through B cell MHC class II molecules: anti-Ia antibodies induce protein kinase C translocation to the nuclear fraction.通过B细胞MHC II类分子的跨膜信号传导:抗Ia抗体诱导蛋白激酶C易位至核部分。
J Immunol. 1987 Apr 1;138(7):2345-52.

II类主要组织相容性复合体分子的平移扩散受其胞质结构域的限制。

Translational diffusion of class II major histocompatibility complex molecules is constrained by their cytoplasmic domains.

作者信息

Wade W F, Freed J H, Edidin M

机构信息

Department of Medicine, National Jewish Center for Immunology and Respiratory Medicine, Denver 80206.

出版信息

J Cell Biol. 1989 Dec;109(6 Pt 2):3325-31. doi: 10.1083/jcb.109.6.3325.

DOI:10.1083/jcb.109.6.3325
PMID:2557353
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2115898/
Abstract

Site-directed mutagenesis in vitro was used to introduce stop codons in the genomic DNA of the alpha and beta chains of the murine class II major histocompatibility complex antigen, I-Ak. Mutated DNA was transfected into B lymphoma cells that were then selected by neomycin resistance and for their ability to express I-Ak molecules on their plasma membrane. The translational diffusion coefficient (Dlat) of I-Ak molecules composed of a wild-type beta chain paired with an alpha chain missing either 6 or 12 amino acids from the cytoplasmic domain is on the average threefold higher than the Dlat of wild-type I-Ak molecules as measured by fluorescence photobleaching and recovery. The removal of 12 amino acids from the cytoplasmic domain of the beta chain did not change the Dlat value from that of wild-type I-Ak if the truncated beta chain was paired with a wild-type alpha chain. Removing all amino acids of the cytoplasmic domains of both the alpha and beta chains resulted in a 10-fold increase in the Dlat, the highest value for any of the truncated I-Ak molecules tested. These data indicate that the carboxy-terminal six amino acids of the cytoplasmic domain of the alpha chain and the six plasma membrane-proximal amino acids of the beta chain are important in constraining the translational diffusion of I-Ak molecules in the plasma membrane.

摘要

体外定点诱变用于在小鼠II类主要组织相容性复合体抗原I-Ak的α链和β链的基因组DNA中引入终止密码子。将突变的DNA转染到B淋巴瘤细胞中,然后通过新霉素抗性及其在质膜上表达I-Ak分子的能力进行筛选。由野生型β链与来自细胞质结构域缺失6个或12个氨基酸的α链配对组成的I-Ak分子的平移扩散系数(Dlat),通过荧光光漂白和恢复测量,平均比野生型I-Ak分子的Dlat高3倍。如果截短的β链与野生型α链配对,从β链的细胞质结构域去除12个氨基酸不会改变其Dlat值,与野生型I-Ak的Dlat值相同。去除α链和β链细胞质结构域的所有氨基酸导致Dlat增加10倍,这是所测试的任何截短的I-Ak分子中的最高值。这些数据表明,α链细胞质结构域的羧基末端六个氨基酸和β链的六个靠近质膜的氨基酸在限制I-Ak分子在质膜中的平移扩散方面很重要。