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设计靶向AML1/MTG8 mRNA的嵌合DNA/RNA锤头状核酶。

Designing of chimeric DNA/RNA hammerhead ribozymes to be targeted against AML1/MTG8 mRNA.

作者信息

Kozu T, Sueoka E, Okabe S, Sueoka N, Komori A, Fujiki H

机构信息

Department of Immunology and Virology, Saitama Cancer Center Research Institute, Japan.

出版信息

J Cancer Res Clin Oncol. 1996;122(4):254-6. doi: 10.1007/BF01209655.

Abstract

For therapeutic purposes, two chimeric DNA/RNA hammerhead ribozymes were synthesized to cleave AML1/MTG8, the t(8;21)-associated fusion mRNA of acute myeloid leukemia. One ribozyme, A/MRZ-1, recognizes the area adjacent to the fusion point between AML1 and MTG8, and cleaves six bases downstream from this point. The other, MRZ-1, recognizes the MTG8 sequence. Both ribozymes cleaved synthetic chimeric DNA/RNA substrates at theoretical sites. Neither cleaved AML1 RNA. A/MRZ-1 cleaved only AML1/MTG8 RNA, and MRZ-1 cleaved both AML1/MTG8 and MTG8 RNAs. The two ribozymes showed growth inhibition of an acute myeloid leukemia cell line carrying t(8;21), SKNO-1 cells. The same extent of growth inhibition was attained by antisense oligonucleotides against AML1/MTG8 RNA. The results suggest that the ribozyme has the potential to be developed as a useful agent for gene therapy, in particular for leukemia with t(8;21).

摘要

为了治疗目的,合成了两种嵌合DNA/RNA锤头状核酶,用于切割急性髓系白血病中与t(8;21)相关的融合mRNA AML1/MTG8。一种核酶A/MRZ-1识别AML1和MTG8之间融合点附近的区域,并在该点下游六个碱基处切割。另一种核酶MRZ-1识别MTG8序列。两种核酶均在理论位点切割合成的嵌合DNA/RNA底物。两者均不切割AML1 RNA。A/MRZ-1仅切割AML1/MTG8 RNA,而MRZ-1切割AML1/MTG8和MTG8 RNA两者。这两种核酶对携带t(8;21)的急性髓系白血病细胞系SKNO-1细胞表现出生长抑制作用。针对AML1/MTG8 RNA的反义寡核苷酸也能达到相同程度的生长抑制。结果表明,核酶有潜力被开发成为一种有用的基因治疗药物,特别是用于治疗t(8;21)白血病。

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Therapeutic antisense and ribozymes.治疗性反义核酸与核酶
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Biological catalysis by RNA.
Annu Rev Biochem. 1986;55:599-629. doi: 10.1146/annurev.bi.55.070186.003123.
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t(8;21) breakpoints on chromosome 21 in acute myeloid leukemia are clustered within a limited region of a single gene, AML1.
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