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对神经生长因子有反应的PC12细胞系不表达Myc二聚化伴侣Max。

The nerve growth factor-responsive PC12 cell line does not express the Myc dimerization partner Max.

作者信息

Hopewell R, Ziff E B

机构信息

Howard Hughes Medical Institute, Department of Biochemistry, New York University Medical Center, New York 10016, USA.

出版信息

Mol Cell Biol. 1995 Jul;15(7):3470-8. doi: 10.1128/MCB.15.7.3470.

Abstract

Heterodimerization of Max with the nuclear oncoprotein Myc and the differentiation-associated proteins Mad and Mxi1 enables these factors to bind E-box sites in DNA and control genes implicated in cell proliferation and differentiation. We show that in the PC12 pheochromocytoma tumor cell line, functional Max protein is not expressed because of the synthesis of a mutant max transcript. This transcript encodes a protein incapable of homo- or heterodimerization. Furthermore, the mutant Max protein, unlike wild-type Max, is incapable of repressing transcription from an E-box element. Synthesis of mutant max transcripts appears to be due to a homozygous chromosomal alteration within the max gene. Reintroduction of max into PC12 cells results in repression of E-box-dependent transcription and a reduction in growth rate, which may explain the loss of Max expression either during the growth of the pheochromocytoma or in subsequent passage of the PC12 cell line in vitro. Finally, the ability of these cells to divide, differentiate, and apoptose in the absence of Max demonstrates for the first time that these processes can occur via Max- and possibly Myc-independent mechanisms.

摘要

Max与核癌蛋白Myc以及与分化相关的蛋白Mad和Mxi1形成异源二聚体,使这些因子能够结合DNA中的E盒位点,并控制与细胞增殖和分化相关的基因。我们发现,在PC12嗜铬细胞瘤肿瘤细胞系中,由于突变型max转录本的合成,功能性Max蛋白未表达。该转录本编码一种无法进行同源或异源二聚化的蛋白质。此外,与野生型Max不同,突变型Max蛋白无法抑制E盒元件的转录。突变型max转录本的合成似乎是由于max基因内的纯合染色体改变。将max重新导入PC12细胞会导致E盒依赖性转录受到抑制,生长速率降低,这可能解释了嗜铬细胞瘤生长过程中或PC12细胞系随后体外传代过程中Max表达缺失的原因。最后,这些细胞在没有Max的情况下进行分裂、分化和凋亡的能力首次证明,这些过程可以通过不依赖Max以及可能不依赖Myc的机制发生。

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