具腦部組織特異表現的蛋白激脢 msbk 基因之選殖與特性分析 Molecular cloning and characterization of a protein kinase msbk
中文摘要我們從老鼠腦部 cDNA 中選殖了一 msbk 基因,與斑馬魚蛋白激脢 bsk146 基因及大鼠 sbk 基因同源,會轉譯出一 417 個胺基酸之 serine/threonine 之蛋白激脢,其 C 端上有一富含有 proline 的區域,內有可和 SH3 ( Src homology 3 ) domain 結合的序列以及具有細胞核定位訊息 ( nuclear locaization signal,NLS ) 的序列,我們構築了 3 種基因片段,msbk-FL ( msbk 基因全長 ) , msbk —KR ( ATP 結合位置變異 ) , sbk—D ( 去 除 C 端 ) 並選殖到 HA-yun 表現載體上,分別去轉染 COS1 、 C6 、 NG108-15 和 HepG2 細胞株,利用免疫染色法,觀察到 mSBK-FL 在 NG108-15 和 HepG2 只會在細胞質表現,在 COS1 和 C6 細胞則是細胞質
和細胞核皆存在, mSBK-KR 及 mSBK-D 就只在細胞質表現,顯示出此蛋白
激脢之表現存在著細胞差異,且推測磷酸化與否及 C 端的 NLS 序列、 SH3 domain 結合序列會影響在細胞中表現的位置。為了進一步分析此基因在生物 體內的功能,我們去選殖出含 msbk 之老鼠基因體片段約 15kb,並將 msbk 之 exon1 置換成 GK-Neo ,製成基因剔除老鼠之目標載體,以便日後生產出 msbk 剔除老鼠;最後我們又選殖出約 5.5kb 之 msbk 5' 端之基因體片 段,利用 pCAT-basic 載體去進行啟動子活性分析,結果顯示啟動子約位在 - 613 ~ + 240 的地方,而在所使用的三種細胞中,以在 NG108-15 中 msbk 啟動子的活性為最強。
英文摘要
We have isolated a mouse gene msbk , which is homologous to zebrafish bsk146 gene and rat sbk gene , from mouse brain cDNA . It encodes a 417 amino acid residues as a serine/threonine protein kinase . It’s C-terminal end contains a proline-rich region , which included a SH3 bind core and a nuclear localization signal ( NLS ) . We have constructed msbk-FL ( wild type msbk ) , msbk-KR ( ATP binding site mutation form ) , msbk-D ( C-terminal end deletion form ) and cloned in HA-yun vector . Then we transfected these plasmids into COS1、C6、NG108-15 and HepG2 cell lines . By immunostaining , we observed that mSBK-FL only expressed in cytoplasm of
NG108-15 and HepG2 cells . But in COS1 and C6 cells , mSBK-FL expressed both in cytoplasm and nucleus . And mSBK-KR and mSBK-D only expressed in cytoplasm of these cell lines. It may reveal that mskb expressed differently in distinct cell lines . And we can guess that phosphorylation and C-terminal end , contained a NLS and SH3 binding core , may affect the cellular localization of mSBK . In order to analyze
the function of msbk in vivo , we also cloned a mouse genomic fragment about 15kb including msbk gene . We replaced the msbk exon1 with GK-Neo . Then we cloned this genomic fragment into a pBSK-sk+ vector to be a targeting vector for msbk knock-out mice . Finally we have cloned a msbk 5’flanking sequence about 5.5 kb . By CAT-basic vector , we performed promoter assay and found that the msbk
promoter was located at -613 ~ +240 . Of these three kinds of cell lines that we used , the msbk promoter activity in NG108 cells was the strongest
