Leprince D, Crepieux P, Stehelin D
INSERM U186/CNRS URA 1160, Institut Pasteur, Lille, France.
Oncogene. 1992 Jan;7(1):9-17.
The proto-oncogene c-ets-1, one of the two cellular sequences transduced by the avian retrovirus E26, encodes for two transcription factors that activate through a purine-rich motif. The v-ets oncogene differs from its cellular progenitor p68c-ets-1 (i) by its fusion to gag- and myb-derived sequences in the E26 P135gag-myb-ets fusion protein, (ii) by two point mutations, and (iii) by the replacement of the 13 C-terminal amino acids present in c-ets-1 by 16 unrelated residues in v-ets. A 35 kDa protein which binds to the purine-rich PEA3 motif in a sequence-specific manner has been obtained by expression in Escherichia coli of the 311 carboxy-terminal amino acids of c-ets-1. Using various v-/c-ets-1 chimeric 35 kDa proteins expressed in bacteria, we have shown that all the mutations found in v-ets, when introduced into this c-ets-1 protein, diminish or even abolish its sequence-specific DNA binding. These results demonstrate that, in addition to the previously defined 85 amino acids located near the carboxy terminus of the c-ets-1 protein (the ETS domain), other sequences are required for sequence-specific DNA binding. In addition, the c-ets-1 35 kDa polypeptide carrying the two point mutations and the viral-specific carboxy terminus, and thus similar to the v-ets-encoded domain of the E26 P135gag-myb-ets, does not bind to the PEA3 motif.
原癌基因c-ets-1是禽逆转录病毒E26转导的两个细胞序列之一,编码两种通过富含嘌呤的基序激活的转录因子。v-ets癌基因与其细胞祖代p68c-ets-1的不同之处在于:(i)在E26 P135gag-myb-ets融合蛋白中与gag和myb衍生序列融合;(ii)存在两个点突变;(iii)v-ets中16个不相关的残基取代了c-ets-1中存在的13个C末端氨基酸。通过在大肠杆菌中表达c-ets-1的311个羧基末端氨基酸,获得了一种以序列特异性方式与富含嘌呤的PEA3基序结合的35 kDa蛋白。利用在细菌中表达的各种v-/c-ets-1嵌合35 kDa蛋白,我们发现,当将v-ets中发现的所有突变引入该c-ets-1蛋白时,会削弱甚至消除其序列特异性DNA结合。这些结果表明,除了先前定义的位于c-ets-1蛋白羧基末端附近的85个氨基酸(ETS结构域)外,序列特异性DNA结合还需要其他序列。此外,携带两个点突变和病毒特异性羧基末端的c-ets-1 35 kDa多肽,因此类似于E26 P135gag-myb-ets的v-ets编码结构域,不与PEA3基序结合。
