Identification of MLL and chimeric MLL gene products involved in 11q23 translocation and possible mechanisms of leukemogenesis by MLL truncation

被引:0
|
作者
Joh, T
Kagami, Y
Yamamoto, K
Segawa, T
Takizawa, J
Takahashi, T
Ueda, R
Seto, M
机构
[1] AICHI CANC CTR, RES INST, LAB CHEMOTHERAPY, CHIKUSA KU, NAGOYA, AICHI 464, JAPAN
[2] AICHI CANC CTR, RES INST, IMMUNOL LAB, CHIKUSA KU, NAGOYA, AICHI 464, JAPAN
[3] AICHI CANC CTR HOSP, DEPT HEMATOL & CHEMOTHERAPY, CHIKUSA KU, NAGOYA, AICHI 464, JAPAN
关键词
translocation; 11q23; MLL; AF9/LTG9; ENL/LTG19; leukemogenesis;
D O I
暂无
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
11q23 chromosome aberrations are frequently observed in infantile as web as therapy-related leukemias, The target gene at 11q23, MLL, is disrupted by the translocation and becomes fused to various translocation partner genes such as AF4/FEL, LTG9/AF9 and LTG19/ENL, The resulting chimeric mRNAs are fused in frame and have been predicted to encode leukemia-specific chimeric proteins, In the present study, we raised antibodies against MLL, LTG9 and LTG19 and demonstrated that MLL and chimeric MLL-LTG9 and MLL-LTG19 products are synthesized in vivo and are localized in the nuclei, using immunofluorescence and cell fractionation studies, The truncated N-terminal portion of the MLL product common to the various types of 11q23 translocation was also localized in the nuclei in a similar fashion, Murine 32Dc13 cells stably expressing the truncated N-terminal MLL protein exhibited an inhibition of differentiation and a growth advantage following stimulation by granulocyte-colony stimulating factor, although the IL-3 dependency was not significantly changed in comparison to the parental cells, These results suggest that the N-terminal portion common to various MLL-chimeric products plays an important role in leukemogenesis.
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页码:1945 / 1953
页数:9
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