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一种针对大鼠大肠表面结肠细胞微绒毛膜的新型标记糖蛋白及其在小肠隐窝细胞中的存在情况。

A novel marker glycoprotein for the microvillus membrane of surface colonocytes of rat large intestine and its presence in small-intestinal crypt cells.

作者信息

Gorr S U, Stieger B, Fransen J A, Kedinger M, Marxer A, Hauri H P

机构信息

Department of Pharmacology, University of Basel, Switzerland.

出版信息

J Cell Biol. 1988 Jun;106(6):1937-46. doi: 10.1083/jcb.106.6.1937.

Abstract

Murine mAbs were produced against purified microvillus membranes of rat colonocytes in order to establish a marker protein for this membrane. The majority of antibodies binding to the colonic microvillus membrane recognized a single protein with a mean apparent Mr of 120 kD in both proximal and distal colon samples. The antigen is membrane bound as probed by phase-partitioning studies using Triton X-114 and by the sodium carbonate extraction procedure and is extensively glycosylated as assessed by endoglycosidase F digestion. Localization studies in adult rats by light and electron microscopy revealed the microvillus membrane of surface colonocytes as the principal site of the immunoreaction. The antigen was not detectable in kidney or liver by immunoprecipitation but was present in the small intestine, where it was predominantly confined to the apical membrane of crypt cells and much less to the microvillus membrane of differentiated enterocytes. During fetal development, the antigen appears first in the colon at day 15 and 1-2 d later in the small intestine. In both segments, it initially covers the whole luminal surface but an adult-like localization pattern develops soon after birth. The antibodies were also used to develop a radiometric assay for the quantification of the antigen in subcellular fractions of colonocytes in order to assess the validity of a previously developed method for the purification of colonic brush-border membranes (Stieger, B., A. Marxer, and H.P. Hauri. 1986. J. Membr. Biol. 91:19-31.). The results suggest that we have identified a valuable marker glycoprotein for the colonic microvillus membrane, which in adult rats may also serve as a marker for early differentiation of enterocyte progenitor cells in small-intestinal crypt cells.

摘要

为了建立大鼠结肠上皮细胞微绒毛膜的标记蛋白,制备了针对纯化的大鼠结肠上皮细胞微绒毛膜的鼠单克隆抗体。在近端和远端结肠样本中,大多数与结肠微绒毛膜结合的抗体识别出一种单一蛋白质,其平均表观分子量为120kD。通过使用Triton X-114的相分离研究和碳酸钠提取程序检测,该抗原与膜结合,并且通过内切糖苷酶F消化评估发现其被广泛糖基化。通过光镜和电镜对成年大鼠进行的定位研究表明,表面结肠上皮细胞的微绒毛膜是免疫反应的主要部位。通过免疫沉淀在肾脏或肝脏中未检测到该抗原,但在小肠中存在,主要局限于隐窝细胞的顶端膜,而在分化的肠上皮细胞的微绒毛膜中含量较少。在胎儿发育过程中,该抗原在第15天首先出现在结肠中,1-2天后出现在小肠中。在这两个节段中,它最初覆盖整个腔表面,但出生后不久就形成了类似成年的定位模式。这些抗体还被用于开发一种放射性测定法,用于定量结肠上皮细胞亚细胞组分中的抗原,以评估先前开发的结肠刷状缘膜纯化方法的有效性(Stieger, B., A. Marxer, and H.P. Hauri. 1986. J. Membr. Biol. 91:19-31.)。结果表明,我们已经鉴定出一种用于结肠微绒毛膜的有价值的标记糖蛋白,在成年大鼠中,它也可以作为小肠隐窝细胞中肠上皮祖细胞早期分化的标记。

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