Coll J, Dozier C, Saule S, Henry C, Quatannens B, Debuire B, Stehelin D
Institut National de la Santé et de la Recherche Médicale U 186, Institut Pasteur de Lille, France.
J Virol. 1988 Aug;62(8):2808-16. doi: 10.1128/JVI.62.8.2808-2816.1988.
The v-mil oncogene of the avian retrovirus MH2 is expressed as a fusion protein with viral gag determinants in infected cells. This P100gag-mil protein accounts for the proliferation of chicken embryo neuroretina cells (CNR) induced by MH2 in vitro. We constructed a series of mutants by in-frame deletions in different parts of the gag and mil domains and tested their ability to induce CNR growth. We show that gag sequences, as well as 200-base-pair 5' mil sequences, were not required to induce such a proliferation. However, gag sequences seem to contribute to a full proliferation of growing CNR. In contrast, deletions in the kinase domain abolish this induction. In particular, by deleting only 9 nucleotides localized around the unique SphI site of v-mil, we produced a totally inactive mutant (BalSp). This mutant directs the synthesis of a v-mil protein lacking the dipeptide Tyr-Leu, which is conserved in almost all the members of the large protein kinase family, and a histidine residue highly conserved in Ser-Thr protein kinase members.
禽逆转录病毒MH2的v-mil癌基因在受感染细胞中表达为一种与病毒gag决定簇融合的蛋白。这种P100gag-mil蛋白导致了MH2在体外诱导鸡胚神经视网膜细胞(CNR)的增殖。我们通过在gag和mil结构域的不同部位进行读框内缺失构建了一系列突变体,并测试了它们诱导CNR生长的能力。我们发现,诱导这种增殖并不需要gag序列以及200个碱基对的5'mil序列。然而,gag序列似乎有助于生长中的CNR的充分增殖。相反,激酶结构域的缺失消除了这种诱导作用。特别是,仅通过缺失v-mil独特的SphI位点周围的9个核苷酸,我们产生了一个完全无活性的突变体(BalSp)。该突变体指导合成一种缺少二肽Tyr-Leu的v-mil蛋白,该二肽在大蛋白激酶家族的几乎所有成员中都是保守的,以及一个在Ser-Thr蛋白激酶成员中高度保守的组氨酸残基。
