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敲除trcp3基因会在小鼠中引发一种隐性神经运动疾病。

Knockout of the trcp3 gene causes a recessive neuromotor disease in mice.

作者信息

Rodríguez-Santiago Magdalena, Mendoza-Torres Merit, Jiménez-Bremont Juan Francisco, López-Revilla Rubén

机构信息

Departamento de Biología Celular, CINVESTAV-IPN, Ap. postal 14-740, 07000 México, D.F., Mexico.

出版信息

Biochem Biophys Res Commun. 2007 Sep 7;360(4):874-9. doi: 10.1016/j.bbrc.2007.06.150. Epub 2007 Jul 6.

DOI:10.1016/j.bbrc.2007.06.150
PMID:17624307
Abstract

Delta202 mice carry a transgene encoding the SV40 T antigen. Mice homozygous for the transgene develop paralysis and atrophy starting at week 4 and die around week 12. To determine the molecular basis of the neurological syndrome, we identified the transgene insertion site by sequencing two successive nested PCR products amplified with reverse primers from circularized Delta202 mouse DNA fragments generated through XbaI digestion. From the cloned products a consensus 542 bp sequence was obtained, with 409 bp corresponding to the transgene ends surrounding a 133 bp sequence formed by a left 128 bp segment and a right 8 bp segment. The 128 bp sequence matched the chr3:36811347-364811421 sequence corresponding to the promoter region of the trpc3 gene between nucleotides -54 and -53 from the transcriptional start point (+1). Complementary DNA amplification from total brain RNA demonstrated a lack of TRPC3 transcripts in Delta202 mouse brain. The neurologic syndrome of Delta202 mice thus appears to be a monogenic recessive neuromotor disease caused by interruption of the trpc3 gene promoter due to the transgene insertion which in turn blocks the transcription and knocks out TRPC3 calcium channels leading to a failure in the postnatal development of the central nervous system.

摘要

Delta202小鼠携带一个编码SV40 T抗原的转基因。该转基因的纯合子小鼠从第4周开始出现麻痹和萎缩,并在第12周左右死亡。为了确定这种神经综合征的分子基础,我们通过对用反向引物从经XbaI消化产生的环化Delta202小鼠DNA片段扩增的两个连续嵌套PCR产物进行测序,确定了转基因插入位点。从克隆产物中获得了一个542 bp的共有序列,其中409 bp对应于转基因末端,围绕着一个由左侧128 bp片段和右侧8 bp片段形成的133 bp序列。该128 bp序列与chr3:36811347 - 364811421序列匹配,该序列对应于trpc3基因启动子区域,位于转录起始点(+1)的核苷酸-54至-53之间。从全脑RNA进行的互补DNA扩增表明Delta202小鼠脑中缺乏TRPC3转录本。因此,Delta202小鼠的神经综合征似乎是一种单基因隐性神经运动疾病,由转基因插入导致trpc3基因启动子中断引起,进而阻断转录并敲除TRPC3钙通道,导致中枢神经系统产后发育失败。

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