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Correct splicing of a group II intron from a chimeric reporter gene transcript in tobacco plastids.

机译:从烟草质体中的嵌合报告基因转录本正确剪接II组内含子。

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摘要

An in vivo test system was developed to study group II intron splicing in higher plant chloroplasts. The chimeric reporter gene uidA was constructed by translational fusion of an intron-containing segment of the plastid atpF gene with the coding region of a plastid uidA reporter gene. The chimeric uidA gene was inserted into the tobacco plastid genome by the biolistic transformation procedure using a plastid targeting vector. Correct intron excision was confirmed by Northern blot analysis, by sequencing amplified cDNAs and by accumulation of the encoded beta-glucuronidase (GUS), the expression of which was dependent on intron removal. Removal of the intron from the uidA mRNA is less efficient (< 50%) than from the atpF mRNA (> 90%). The efficiency of atpF mRNA splicing is not affected in the plasmid transformants indicating that inefficient splicing of the highly-expressed uidA mRNA is not due to depletion of factor(s) required for the atpF intron removal. A derivative of uidA, with a stop codon introduced into the loop of domain VI, was also tested. The mutations did not affect the splicing efficiency. The chimeric uidA splicing system will facilitate the study of structural and sequence requirements for group II intron splicing in plastids of higher plants.
机译:开发了一种体内测试系统来研究高等植物叶绿体中的II组内含子剪接。嵌合报告基因uidA是通过质体atpF基因的含内含子的片段与质体uidA报告基因的编码区的翻译融合而构建的。通过使用质体靶向载体的生物射弹转化方法将嵌合uidA基因插入到烟草质体基因组中。通过Northern印迹分析,测序扩增的cDNA和积累编码的β-葡萄糖醛酸苷酶(GUS)证实了正确的内含子切除,其表达取决于内含子的去除。从uidA mRNA去除内含子的效率(<50%)比从atpF mRNA去除(> 90%)的效率低。 atpF mRNA剪接的效率在质粒转化体中不受影响,这表明高表达的uidA mRNA的剪接效率低不是由于耗尽了atpF内含子所需的因子的消耗所致。还测试了uidA的衍生物,其终止密码子引入域VI的环中。突变不影响剪接效率。嵌合的uidA剪接系统将有助于研究高等植物质体中II组内含子剪接的结构和序列要求。

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