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蟾蜍膀胱上皮细胞顶端膜和基底外侧膜的差异共价标记

Differential covalent labeling of apical and basal-lateral membranes of the epithelium of the toad bladder.

作者信息

Ekblad E B, Strum J M, Edelman I S

出版信息

J Membr Biol. 1976 Mar 18;26(2-3):301-17. doi: 10.1007/BF01868879.

Abstract

The apical (luminal) plasma membrane of toad bladder epithelial cells has been labeled with (125I) diazo-diiodo sulfanilic acid (125I-DDISA) as demonstrated by electron-microscopic autoradiography. The silver grains (125I) were localized exclusively to the apical surface. At concentrations of DDISA of 10(-3) M or less, binding to the apical membrane had no significant effect on the fine structure of the epithelium. At concentrations of DDISA of 10(-6) M or less, the baseline short-circuit current (SCC), and the response to cyclic 3',5'-adenosine monophosphate (cAMP) plus theophylline were unimpaired. At 10(-5) M, baseline SCC was unchanged and the response to cyclic AMP plus theophylline was enhanced. At concentrations of 10(-4) M and greater baseline SCC was depressed and the response to the nucleotide inhibited. The basal-lateral epithelial plasma membranes were labeled by exposing the serosal side to pyridoxal phosphate and reducing the resultant Schiff base with sodium borotritide (3H-NaBH1). In electron-microscopic autoradiographs, the silver grains (3H) were found over the basal and lateral surfaces of the epithelium. At concentrations of pyridoxal phosphate of 10(-4) M and 3H-NaBH1 of 10(-3) M, there were no significant changes in the fine structure of the epithelium. Addition of pyridoxal phosphate (10(-4) M) and NaBH4 (10(-3) M) to the serosal side decreased the baseline SCC significantly but not the response to vasopressin. Covalent attachment of the 125I and the 3H was indicated by resistance to elution in the preparation of the sections for electron-microscopy and the reagent requirements for binding.

摘要

通过电子显微镜放射自显影法证明,蟾蜍膀胱上皮细胞的顶端(管腔)质膜已用(125I)重氮二碘磺胺酸(125I-DDISA)标记。银颗粒(125I)仅定位于顶端表面。在DDISA浓度为10^(-3)M或更低时,与顶端膜的结合对上皮细胞的精细结构无显著影响。在DDISA浓度为10^(-6)M或更低时,基线短路电流(SCC)以及对环3',5'-腺苷单磷酸(cAMP)加茶碱的反应未受损害。在10^(-5)M时,基线SCC不变,对环AMP加茶碱的反应增强。在浓度为10^(-4)M及更高时,基线SCC降低,对核苷酸的反应受到抑制。通过将浆膜侧暴露于磷酸吡哆醛并用硼氢化三钠(3H-NaBH4)还原所得席夫碱来标记基底-外侧上皮细胞质膜。在电子显微镜放射自显影片中,银颗粒(3H)出现在上皮细胞的基底和外侧表面。在磷酸吡哆醛浓度为10^(-4)M和3H-NaBH4浓度为10^(-3)M时,上皮细胞的精细结构无显著变化。向浆膜侧添加磷酸吡哆醛(10^(-4)M)和硼氢化钠(10^(-3)M)可显著降低基线SCC,但不影响对血管加压素的反应。在制备用于电子显微镜检查的切片时,125I和3H的抗洗脱性以及结合所需的试剂表明它们发生了共价连接。

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