Brunner S, Kramar K, Denhardt D T, Hofbauer R
Institut für Molekularbiologie, Wiener Biozentrum, Universität Wien, Austria.
Biochem J. 1997 Mar 1;322 ( Pt 2)(Pt 2):403-10. doi: 10.1042/bj3220403.
We have employed a newly developed differential screening technique (reverse strand priming) to identify murine carnitine acetyltransferase (CARAT) as a growth- and cell cycle-regulated gene in S3T3 mouse fibroblasts. Sequence analysis of the full-length cDNA clone and homology comparisons have revealed 87% homology to the human CARAT gene. On Northern blots we were able to measure a 2-3-fold induction 18 h after a mitogenic stimulus following serum deprivation as well as after release from a sodium butyrate block. The cell cycle induction pattern of the CARAT gene was analysed in mouse fibroblasts at different stages of the unperturbed cell cycle. Fractions obtained by elutriation of an exponentially growing culture showed a biphasic maximum of transcript abundance in the G1 and G2 phases of the cell cycle. CARAT expression was investigated in several organs of the adult mouse. Among those measured, CARAT expression was highest, relative to liver, in heart muscle (56-fold) and testis (21-fold). Using both conventional antisense oligodeoxynucleotides and novel single-stranded antisense phagemid DNA, we obtained evidence that the CARAT enzyme function is necessary for progression through G1 and into the S-phase of the cell cycle.
我们采用了一种新开发的差异筛选技术(反向链引发),以鉴定小鼠肉碱乙酰转移酶(CARAT)是S3T3小鼠成纤维细胞中一种受生长和细胞周期调控的基因。对全长cDNA克隆的序列分析和同源性比较显示,它与人类CARAT基因有87%的同源性。在Northern印迹分析中,我们能够检测到在血清剥夺后的促有丝分裂刺激18小时后,以及从丁酸钠阻断中释放后,CARAT基因有2至3倍的诱导。我们在未受干扰的细胞周期不同阶段的小鼠成纤维细胞中分析了CARAT基因的细胞周期诱导模式。通过淘洗指数生长的培养物获得的细胞组分显示,在细胞周期的G1期和G2期转录本丰度有双相最大值。我们在成年小鼠的多个器官中研究了CARAT的表达。在所检测的器官中,相对于肝脏,CARAT在心肌(56倍)和睾丸(21倍)中的表达最高。使用传统的反义寡脱氧核苷酸和新型单链反义噬菌粒DNA,我们获得了证据,证明CARAT酶功能对于细胞周期从G1期进入S期的进程是必需的。
