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用细胞松弛素B进行光亲和标记鉴定猴晶状体葡萄糖转运体

Identification of the monkey lens glucose transporter by photoaffinity labelling with cytochalasin B.

作者信息

Lucas V A, Zigler J S

机构信息

Laboratory of Mechanisms of Ocular Diseases, National Eye Institute, Bethesda, Maryland.

出版信息

Invest Ophthalmol Vis Sci. 1988 Apr;29(4):630-5.

PMID:3128491
Abstract

Polypeptide constituents of the lens glucose transporter have been identified by photoaffinity labelling with cytochalasin B. The urea-insoluble fraction of monkey lens was irradiated at 280 nm for 30 min in the presence of 5 X 10(-7) M 3H-cytochalasin B. After extensive washing, the membranes were solubilized and their polypeptide composition determined by SDS-PAGE. Radioactivity was extracted from gel slices to determine the position of photoincorporated label. 3H-cytochalasin B was irreversibly incorporated into a broad molecular weight region from Mr greater than 94,000 to 43,000 with the peak of activity occurring at Mr 53,000. Photoincorporation was inhibited by D-glucose (500 mM) and phloretin (1 X 10(-5] but was unaffected by L-glucose (500 mM), cytochalasin E (1 X 10(-5) and phloridzin (1 X 10(-5) M). Cortex and nucleus membrane preparations contained the same range of labelled polypeptides after photoaffinity labelling but nuclear membranes contained approximately twice the activity of cortical membranes indicating an enrichment of glucose transporters in the nucleus. Treatment of labelled membranes with endoglycosidase F converted the broad band of labelling to a sharp band of Mr 45,000. The lens glucose transporter is therefore a glycoprotein and the broadness of the photaffinity labelled peak is due to heterogeneous N-linked glycosylation of a core polypeptide. From these studies it appears that the monkey lens glucose transporter closely resembles that of the human erythrocyte.

摘要

通过用细胞松弛素B进行光亲和标记,已鉴定出晶状体葡萄糖转运蛋白的多肽成分。在5×10⁻⁷M³H-细胞松弛素B存在的情况下,将猴晶状体的尿素不溶部分在280nm下照射30分钟。经过充分洗涤后,将膜溶解,并通过SDS-PAGE测定其多肽组成。从凝胶切片中提取放射性以确定光掺入标记的位置。³H-细胞松弛素B不可逆地掺入分子量范围从大于94,000到43,000的宽区域,活性峰值出现在Mr 53,000处。光掺入受到D-葡萄糖(500mM)和根皮素(1×10⁻⁵)的抑制,但不受L-葡萄糖(500mM)、细胞松弛素E(1×10⁻⁵)和根皮苷(1×10⁻⁵M)的影响。光亲和标记后,皮质和核膜制剂含有相同范围的标记多肽,但核膜的活性约为皮质膜的两倍,表明核中葡萄糖转运蛋白富集。用内切糖苷酶F处理标记的膜将宽的标记带转化为Mr 45,000的尖锐带。因此,晶状体葡萄糖转运蛋白是一种糖蛋白,光亲和标记峰的宽度是由于核心多肽的异质性N-连接糖基化。从这些研究看来,猴晶状体葡萄糖转运蛋白与人类红细胞的非常相似。

相似文献

1
Identification of the monkey lens glucose transporter by photoaffinity labelling with cytochalasin B.用细胞松弛素B进行光亲和标记鉴定猴晶状体葡萄糖转运体
Invest Ophthalmol Vis Sci. 1988 Apr;29(4):630-5.
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Transmembrane glucose carriers in the monkey lens. Quantitation and regional distribution as determined by cytochalasin B binding to lens membranes.
Invest Ophthalmol Vis Sci. 1987 Aug;28(8):1404-12.
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Photoaffinity labeling of the K562 cell membrane D-glucose transporter with cytochalasin B.用细胞松弛素B对K562细胞膜D-葡萄糖转运体进行光亲和标记。
Biochem Int. 1986 Feb;12(2):199-206.
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Photoaffinity labeling of the stereospecific D-glucose transport system with cytochalasin B.用细胞松弛素B对立体特异性D-葡萄糖转运系统进行光亲和标记。
Fed Proc. 1984 May 15;43(8):2258-61.
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Identification of glucose and nucleoside transport proteins in neonatal pig erythrocytes using monoclonal antibodies against band 4.5 polypeptides of adult human and pig erythrocytes.利用抗成人及猪红细胞4.5带多肽的单克隆抗体鉴定新生猪红细胞中的葡萄糖和核苷转运蛋白。
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Identification and characterization of the glucose-transport protein of the bovine blood/brain barrier.牛血脑屏障葡萄糖转运蛋白的鉴定与特性分析
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[Quantitative autoradiography of the glucose transport protein with (3H)cytochalasin-B in the mammalian eye].
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Cytochalasin B does not serve as a marker of glucose transport in rabbit erythrocytes.细胞松弛素B不能作为兔红细胞葡萄糖转运的标志物。
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Solubilization and separation of the human erythrocyte D-glucose transporter covalently and noncovalently photoaffinity-labeled with [3H]cytochalasin B.用[3H]细胞松弛素B对人红细胞D-葡萄糖转运体进行共价和非共价光亲和标记后的增溶与分离。
Proc Natl Acad Sci U S A. 1986 Jan;83(2):479-82. doi: 10.1073/pnas.83.2.479.
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Chemical identity of the glucose transporter with the [3H]cytochalasin B-photolabelled component of human erythrocyte membranes. Equal sensitivity to trypsin and endoglycosidase F.葡萄糖转运蛋白与人类红细胞膜上[3H]细胞松弛素B光标记成分的化学特性。对胰蛋白酶和内切糖苷酶F的敏感性相同。
Biochem Biophys Res Commun. 1984 Jul 18;122(1):218-24. doi: 10.1016/0006-291x(84)90462-5.

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