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二氟甲基鸟氨酸抗性细胞系DH23b中稳定型鸟氨酸脱羧酶和抗酶的过量产生。

Overproduction of stable ornithine decarboxylase and antizyme in the difluoromethylornithine-resistant cell line DH23b.

作者信息

Mitchell J L, Choe C Y, Judd G G, Daghfal D J, Kurzeja R J, Leyser A

机构信息

Department of Biological Sciences, Northern Illinois University, DeKalb 60115, USA.

出版信息

Biochem J. 1996 Aug 1;317 ( Pt 3)(Pt 3):811-6. doi: 10.1042/bj3170811.

Abstract

DH23b cells, a variant of the HTC line selected for their resistance to difluoromethylornithine, exhibit defective feedback regulation of ornithine decarboxylase (ODC) stability and polyamine transport, and accumulate ODC protein to > 1000 times normal concentrations. The components of the polyamine feedback regulation system have been examined in an attempt to understand these unusual responses. Southern-blot analysis revealed an amplification (approx. 10-fold) in ODC DNA sequence without any concomitant increase in antizyme. Moreover, the amplified ODC sequence contains a single base substitution that results in the conversion of Cys-441 into Trp. This modification has previously been shown to cause ODC stability in HMOA cells. Although antizyme activity has not been noted in DH23b cells, Western-blot analysis revealed the accumulation of antizyme protein to > 50 times that induced in parental HTC cells. This increase is consistent with a 6-9-fold increase in the half-life of antizyme in these cells, a consequence of the inability of the mutant ODC-antizyme complex to be degraded by 26 S proteasome. Associated with the stabilization of antizyme in both DH23b and HMOA cells is the appearance of two additional forms of antizyme protein with apparent molecular masses of 22 and 18.5 kDa. It is suggested that these result from proteolytic removal of discrete fragments from the N-terminal end of antizyme, perhaps an indication of an initial step in rapid antizyme turnover.

摘要

DH23b细胞是HTC细胞系的一个变体,因其对二氟甲基鸟氨酸具有抗性而被筛选出来,该细胞系鸟氨酸脱羧酶(ODC)稳定性和多胺转运的反馈调节存在缺陷,ODC蛋白积累至正常浓度的1000倍以上。为了理解这些异常反应,对多胺反馈调节系统的组成成分进行了研究。Southern印迹分析显示ODC DNA序列有扩增(约10倍),而抗酶没有相应增加。此外,扩增的ODC序列包含一个单碱基取代,导致Cys-441转变为Trp。先前已证明这种修饰会导致HMOA细胞中ODC的稳定性。虽然在DH23b细胞中未观察到抗酶活性,但Western印迹分析显示抗酶蛋白积累至亲本HTC细胞诱导水平的50倍以上。这种增加与这些细胞中抗酶半衰期增加6 - 9倍一致,这是突变型ODC - 抗酶复合物无法被26S蛋白酶体降解的结果。与DH23b和HMOA细胞中抗酶的稳定化相关的是出现了另外两种抗酶蛋白形式,表观分子量分别为22 kDa和18.5 kDa。推测这是由于抗酶N末端离散片段的蛋白水解去除所致,这可能是抗酶快速周转初始步骤的一个指示。

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