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突变早老素1和2导致中国仓鼠卵巢细胞内β淀粉样蛋白42水平升高的不同机制。

Distinct mechanisms by mutant presenilin 1 and 2 leading to increased intracellular levels of amyloid beta-protein 42 in Chinese hamster ovary cells.

作者信息

Qi Yue, Morishima-Kawashima Maho, Sato Toru, Mitsumori Rie, Ihara Yasuo

机构信息

Department of Neuropathology, Faculty of Medicine, University of Tokyo, 7-3-1 Hongo, Bunkyo-ku, Tokyo 113-0033, Japan.

出版信息

Biochemistry. 2003 Feb 4;42(4):1042-52. doi: 10.1021/bi0267590.

Abstract

To characterize the properties of presenilin (PS) 1- and PS2-associated gamma-secretases, we established stable transfectants overexpressing amyloid precursor protein and wild-type (wt) or a number of mutant (mt) PS1 or PS2. Quantification of the intracellular amyloid beta-protein (Abeta) levels in mtPS1 and mtPS2 cell lines revealed the presence of two subtypes. One group consists of N141I, M239V, and T122P mutations of the PS2 gene and homologous mutations of PS1, N135D and M233T. These mutations led to an increase in the intracellular Abeta42 levels and a concomitant decrease in the intracellular Abeta40 levels. A cell-free assay for Abeta production using the membranes prepared from these transfectants exhibited predominant cleavage at position Abeta42 with marginal production of Abeta40. The other group consists of M146L, H163R, and G384A mutations of PS1, leading only to an increase in the intracellular Abeta42 levels. While the intracellular Abeta levels in M146L cells were consistent with the results from cell-free Abeta production, H163R and G384A cells showed significant discrepancies between the intracellular Abeta levels and cell-free Abeta production. Thus, all the mtPS1/2 examined here result in increases in the intracellular Abeta42 levels. This suggests that the underlying mechanisms for this shared phenotype may be diverse.

摘要

为了描述早老素(PS)1和PS2相关γ-分泌酶的特性,我们建立了稳定转染细胞系,这些细胞系过表达淀粉样前体蛋白以及野生型(wt)或多种突变型(mt)的PS1或PS2。对mtPS1和mtPS2细胞系中细胞内淀粉样β蛋白(Aβ)水平的定量分析揭示了两种亚型的存在。一组包括PS2基因的N141I、M239V和T122P突变以及PS1的同源突变N135D和M233T。这些突变导致细胞内Aβ42水平升高,同时细胞内Aβ40水平降低。使用从这些转染细胞制备的膜进行的Aβ产生的无细胞测定显示,在Aβ42位点有主要切割,Aβ40产生较少。另一组包括PS1的M146L、H163R和G384A突变,仅导致细胞内Aβ42水平升高。虽然M146L细胞中的细胞内Aβ水平与无细胞Aβ产生的结果一致,但H163R和G384A细胞在细胞内Aβ水平和无细胞Aβ产生之间显示出显著差异。因此,这里检测的所有mtPS1/2都导致细胞内Aβ42水平升高。这表明这种共同表型的潜在机制可能多种多样。

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