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大鼠腮腺腺泡细胞中rab护送蛋白亚型的表达与定位

Expression and localization of rab escort protein isoforms in parotid acinar cells from rat.

作者信息

Chan D, Lin J, Raffaniello R D

机构信息

Division of Digestive Diseases, Department of Medicine, State University of New York-Health Science Center at Brooklyn, Brooklyn, New York, USA.

出版信息

J Cell Physiol. 2000 Dec;185(3):339-47. doi: 10.1002/1097-4652(200012)185:3<339::AID-JCP4>3.0.CO;2-4.

Abstract

Rab proteins are geranylgeranylated on their carboxyl terminal cysteine motifs by geranylgeranyltransferase II (GGTase). Rab escort protein (REP) is required to present Rab proteins to GGTase. REP may remain bound to newly isoprenylated Rab proteins and present them to their target membrane. Other studies have shown that Rab proteins cycle between the membrane and cytosolic compartments and that cytosolic Rab proteins are complexed with rab-GDI. In the present study, we examined the expression and localization of REP isoforms in parotid acinar cells. Although both REP isoforms, REP-1 and REP-2, were detected in parotid cytosol, REP-2 was the predominant isoform. Subcellular fractionation revealed that approximately 42% of cellular REP-2 is membrane-associated. REP-2 was partially removed from parotid membranes with 1 M NaCl or Na(2)CO(3), indicating that REP-2 is a peripheral membrane protein. Membrane-associated REP-2 did not colocalize with Rab3D on secretory granule membranes. However, density gradient centrifugation revealed that membrane-associated REP-2 and Rab3D colocalize on low- and high-density membrane fractions in parotid acinar cells. Isoproterenol, an agent which induces amylase release from parotid glands, caused a shift in both REP-2 and Rab3D to less dense membrane fractions. When acinar cell cytosol was fractionated by gel filtration chromatography, Rab3D eluted exclusively with REP, not rab-GDI. In contrast, Rab1B and Rab5 eluted with both REP and Rab-GDI. Colocalization of Rab3D and REP-2 on acinar cell membranes suggests that REP-2 plays a role in delivering Rab3D to parotid membranes and may regulate guanine nucleotide binding to membrane-associated Rab3D. In addition, unlike other Rab proteins, cytosolic Rab3D appears to associate exclusively with REP, not rab-GDI in parotid acinar cells.

摘要

Rab蛋白通过香叶基香叶基转移酶II(GGTase)在其羧基末端半胱氨酸基序上进行香叶基香叶基化修饰。Rab护送蛋白(REP)是将Rab蛋白呈递给GGTase所必需的。REP可能会与新异戊二烯化的Rab蛋白保持结合,并将它们呈递给其靶膜。其他研究表明,Rab蛋白在膜和胞质区室之间循环,并且胞质Rab蛋白与rab - GDI形成复合物。在本研究中,我们检测了腮腺腺泡细胞中REP亚型的表达和定位。尽管在腮腺胞质溶胶中检测到了两种REP亚型,即REP - 1和REP - 2,但REP - 2是主要亚型。亚细胞分级分离显示,约42%的细胞REP - 2与膜相关。用1 M NaCl或Na₂CO₃可从腮腺膜中部分去除REP - 2,这表明REP - 2是一种外周膜蛋白。膜相关的REP - 2在分泌颗粒膜上不与Rab3D共定位。然而,密度梯度离心显示,膜相关的REP - 2和Rab3D在腮腺腺泡细胞的低密度和高密度膜组分中共定位。异丙肾上腺素是一种诱导腮腺淀粉酶释放的物质,它导致REP - 2和Rab3D都向密度较低的膜组分转移。当通过凝胶过滤色谱法对腺泡细胞胞质溶胶进行分级分离时,Rab3D仅与REP一起洗脱,而不与rab - GDI一起洗脱。相反,Rab1B和Rab5与REP和Rab - GDI一起洗脱。Rab3D和REP - 2在腺泡细胞膜上的共定位表明,REP - 2在将Rab3D递送至腮腺膜中发挥作用,并且可能调节鸟嘌呤核苷酸与膜相关Rab3D的结合。此外,与其他Rab蛋白不同,在腮腺腺泡细胞中,胞质Rab3D似乎仅与REP结合,而不与rab - GDI结合。

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