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植物回收蛋白定位于拟南芥的液泡前体区室和微泡中,可能与液泡分选受体相互作用。

Plant retromer, localized to the prevacuolar compartment and microvesicles in Arabidopsis, may interact with vacuolar sorting receptors.

作者信息

Oliviusson Peter, Heinzerling Oliver, Hillmer Stefan, Hinz Giselbert, Tse Yu Chung, Jiang Liwen, Robinson David G

机构信息

Department of Cell Biology, Heidelberg Institute for Plant Sciences, University of Heidelberg, 69120 Heidelberg, Germany.

出版信息

Plant Cell. 2006 May;18(5):1239-52. doi: 10.1105/tpc.105.035907. Epub 2006 Mar 31.

Abstract

Receptors for acid hydrolases destined for the lytic compartment in yeast and mammalian cells are retrieved from intermediate, endosomal organelles with the help of a pentameric protein complex called the retromer. We cloned the Arabidopsis thaliana homologs of the three yeast proteins (Vps35, Vps29, and Vps26) constituting the larger subunit of retromer and prepared antisera against them. With these antibodies, we demonstrated the presence of a retromer-like protein complex in salt extracts prepared from Arabidopsis microsomes. This complex is associated with membranes that coequilibrate with prevacuolar compartment markers and with high-density sedimenting membranes. Immunogold negative staining identified these membranes as 90-nm-diameter coated microvesicles. Confocal laser scanning immunofluorescence studies performed on tobacco (Nicotiana tabacum) BY-2 cells revealed high degrees of colabeling between all three retromer antisera and the prevacuolar compartment (PVC) markers PEP12 and vacuolar sorting receptor VSR(At-1). The presence of plant retromer at the surface of multivesicular bodies was also demonstrated by immunogold labeling of sections obtained from high-pressure frozen/freeze-substituted specimens. Treatment of BY-2 cells with wortmannin led to swelling of the PVC and a separation of the VPS35 and VSR signals. Preliminary data suggesting that retromer interacts with the cytosolic domain of a VSR were obtained by immunoprecipitation experiments performed on detergent-solubilized microsomes with Vps35 antibodies.

摘要

在酵母和哺乳动物细胞中,前往溶酶体区室的酸性水解酶的受体借助一种名为回收体的五聚体蛋白复合物从中级内体细胞器中回收。我们克隆了构成回收体较大亚基的三种酵母蛋白(Vps35、Vps29和Vps26)的拟南芥同源物,并制备了针对它们的抗血清。利用这些抗体,我们证明了在从拟南芥微粒体制备的盐提取物中存在一种类似回收体的蛋白复合物。这种复合物与与液泡前体区室标记物共平衡的膜以及高密度沉降膜相关。免疫金负染色将这些膜鉴定为直径90纳米的被膜微泡。对烟草(Nicotiana tabacum)BY - 2细胞进行的共聚焦激光扫描免疫荧光研究显示,所有三种回收体抗血清与液泡前体区室(PVC)标记物PEP12和液泡分选受体VSR(At - 1)之间存在高度共标记。通过对高压冷冻/冷冻置换标本切片的免疫金标记,也证明了多泡体表面存在植物回收体。用渥曼青霉素处理BY - 2细胞会导致PVC肿胀以及VPS35和VSR信号分离。通过用Vps35抗体对去污剂溶解的微粒体进行免疫沉淀实验,获得了初步数据,表明回收体与VSR的胞质结构域相互作用。

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