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小鼠釉原蛋白[A-4]/M59细胞表面受体的特性分析

Characterization of a mouse amelogenin [A-4]/M59 cell surface receptor.

作者信息

Tompkins Kevin, George Anne, Veis Arthur

机构信息

Department of Cell and Molecular Biology, Northwestern University Feinberg School of Medicine, 303 E. Chicago Ave Ward-13-100 Chicago, IL 60611, USA.

出版信息

Bone. 2006 Feb;38(2):172-80. doi: 10.1016/j.bone.2005.08.013. Epub 2005 Oct 6.

Abstract

Amelogenin proteins comprise up to 90% of the organic matrix of developing enamel in the vertebrate tooth. Alternative splicing of mouse amelogenin pre-mRNA leads to the production of more than 14 protein isoforms, the functions of which are not totally understood. The smaller splice products, [A + 4] or M73 and [A - 4] or M59, have been shown to act differently as signaling molecules affecting odontogenic and other cell types. The mechanisms of these signaling processes, beginning with receptor identification, are not well understood. Utilizing radiolabeled [A - 4], we show here that 3H[A - 4] binds in a saturable fashion to the cell surface of C2C12 mouse fetal myoblasts at 4 degrees C, and not only binds at the surface but is internalized at 37 degrees C. "Far Western" immunohistochemistry performed on sections of E18 mouse incisors and molars with biotin-labeled [A - 4] as the primary ligand demonstrates [A - 4]-biotin binding to polarizing ameloblasts and odontoblasts, cells of the dental follicle, and along the stratum intermedium. Using [A - 4] affinity column chromatography and [A - 4]-biotin label transfer reaction, we have identified a 95 kDa C2C12 cell surface protein which bound [A - 4]. Utilizing Tandem MS (MS/MS) sequencing, we report the novel finding of the 95 kDa murine transmembrane protein, LAMP-1, originally identified as a lysosomal membrane protein that is also found at the cell surface, as an [A - 4] cell binding protein.

摘要

釉原蛋白占脊椎动物牙齿发育中釉质有机基质的90%。小鼠釉原蛋白前体mRNA的可变剪接产生了14种以上的蛋白质异构体,其功能尚未完全明确。较小的剪接产物,[A + 4]或M73以及[A - 4]或M59,已被证明作为影响牙源性和其他细胞类型的信号分子,其作用方式不同。从受体识别开始的这些信号传导过程的机制尚不清楚。利用放射性标记的[A - 4],我们在此表明3H[A - 4]在4℃下以可饱和的方式与C2C12小鼠胎儿成肌细胞的细胞表面结合,不仅在表面结合,而且在37℃下内化。用生物素标记的[A - 4]作为主要配体,对E18小鼠切牙和磨牙切片进行“Far Western”免疫组织化学,结果显示[A - 4]-生物素与极化的成釉细胞、成牙本质细胞、牙囊细胞以及中间层结合。利用[A - 4]亲和柱色谱和[A - 4]-生物素标记转移反应,我们鉴定出一种与[A - 4]结合的95 kDa C2C12细胞表面蛋白。利用串联质谱(MS/MS)测序,我们报告了一个新发现,即95 kDa的小鼠跨膜蛋白LAMP-1,最初被鉴定为一种溶酶体膜蛋白,也存在于细胞表面,它是一种[A - 4]细胞结合蛋白。

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