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Construction and Expression of Vector with aroA-In Gene and Its Transformation in Tobacco

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ã€Authorã€‘ ZHAO Jin,GAO Su-Qin,FEI Yun-Biao,WEI Ling-Bo~â‘ (Institute of Genetics and Developmental Biology ,Chinese Academy of Sciences ,Beijing 100080,China)

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ã€æ‘˜è¦ã€‘ PCRæ‰©å¢žçªå˜çš„ 5â€² çƒ¯é†‡ä¸™é…®é…¸èŽ½è‰é…¸ 3 ç£·é…¸åˆæˆé…¶ (5â€² enolpyruvylshikimate 3 phosphatesynthetase ,EPSPS)cDNAå…¨é•¿åºåˆ— ,æ’å…¥ pLitmus2 8å¾—åˆ° pLEPSPS ,è¿›è€Œé€šè¿‡åå‘PCRåœ¨EPSPS 2 35 /2 36aaä¹‹é—´å°†å…¶æ‰“æ–ä¸ºæ— åŠŸèƒ½çš„ç‰‡æ®µã€‚é€‰ç”¨äººå·¥æž„å»ºçš„å…·æœ‰é¡ºå¼å’Œåå¼å‰ªæŽ¥åŠŸèƒ½çš„miniåž‹è›‹ç™½å†…å«åSspDnaBå’ŒRmaDnaB ,æ’å…¥è¢«æ‰“æ–çš„aroA(æŠ—é™¤è‰å‰‚åŸºå› ) ,æž„å»ºäº†è´¨ç²’ pLEBCã€pLEBTã€pLERCå’Œ pLERTã€‚å°† 4ç§é‡ç»„è´¨ç²’ä¸çš„aroA In(è›‹ç™½å†…å«åInteinæ’å…¥aroA)èžåˆåŸºå› æ’å…¥ pET 32å¾—åˆ°è¡¨è¾¾è½½ä½“ pETLEBCã€pETLEBTã€pETLERCå’Œ pETLERT ,IPTGè¯±å¯¼åŽ ,SDS PAGEåˆ†æžæ˜¾ç¤ºå…¶èƒ½åœ¨DE3 ä¸æœ‰æ•ˆè¡¨è¾¾å¹¶å‘ç”Ÿç›¸åº”çš„è›‹ç™½å‰ªæŽ¥ã€‚å°†aroA cisSspDnaBå’ŒaroA cisRmaDnaBèžåˆåŸºå› åˆ†åˆ«æ’å…¥ pLYMä¸è¿›ä¸€æ¥æž„å»ºæˆæ¤ç‰©è¡¨è¾¾è½½ä½“ ,å†œæ†èŒå¶ç›˜æ³•è½¬åŒ–çƒŸè‰ã€‚åŸºå› ç»„PCRåˆ†æžè¡¨æ˜ŽèžåˆåŸºå› æ•´åˆå…¥æ¤ç‰©æ ¸åŸºå› ç»„ ;RT PCRåˆ†æžæ˜¾ç¤ºå…¶å¯åœ¨é«˜ç‰æ¤ç‰©ç»†èƒžä¸æˆåŠŸè¡¨è¾¾ã€‚ç»“æžœè¯´æ˜Žè›‹ç™½å†…å«ååŸºå› å¯ä»¥è½¬åŒ–é«˜ç‰çœŸæ ¸ç»†èƒž ,è›‹ç™½å‰ªæŽ¥æŠ€æœ¯å¯åº”ç”¨äºŽé«˜ç‰æ¤ç‰©ç»†èƒž ,ä»Žè€Œä¸ºé˜²æ¢æ¤ç‰©è½¬åŸºå› æ‰©æ•£æä¾›äº†ä¸€æ¡æ–°çš„é€”å¾„æ›´å¤š è¿˜åŽŸ

ã€Abstractã€‘ Inteins are intervening protein sequences that undergo self-excision from precursor protein with concomitant joining of flanking sequences. Here,we demonstrated intein cis-splicing in Nicotiana tabacum nuclear genomes by using artificial cis Ssp DnaB and Rma DnaB intein.We want to test whether protein splicing can occur in higher eucaryotic cell,which would play an important role in transgene containment in transgenic plants.Glyphosate-resistant Salmonella typhimurium aroA gene was divided at position 235/236 aa within EPSPS by inverse PCR from pLEPSPS. Amplified gene products with artificial cis-Ssp DnaB/Rma DnaB intein and split-Ssp DnaB/Rma DnaB intein were inserted at position 235 of EPSPS respectively to construct plasmid pLEBC,pLERC,pLEBT and pLERT.Above four aroA-In gene fusions were ligated into pET-32 to obtain E.coli expression vectors termed pETLEBC,pETLEBT,pETLERC and pETLERT.E.coli DE₃ cells containing individual recombinant plasmids described above were induced by IPTG to produce corresponding protein products.Detectable spliced EPSPS and unspliced precursor demonstrated that splicing occurred in bacteria. aroA-cis SSp DnaB and aroA-cis Rma DnaB were ligated into Agrobacterium tumefaciens binary vector pLYM. Then A.tumefaciens containing EPSPS-ï¼ˆcisï¼‰ intein cassettes were used for leaf disk transformation in N.tabacum.Integration of aroA-In gene into plant genome was confirmed by genomic PCR analyses. To verify the expression of fusion genes at transcriptional level,RT-PCR analyses were performed and the expected products were identified.These results suggested that plant cells support expression of S.typhimurium aroA-In fusion gene in nulear genomes.Thus,we speculated the existence of protein-splicing activity in plant cells.This opens the possibility of applying intein trans-splicing technique to reduce/prevent gene transfer by way of pollen in transgenic plants.æ›´å¤š è¿˜åŽŸ

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ã€Key wordsã€‘ protein splicingï¼› EPSPSï¼› genetic transformationï¼› Nicotiana tabacumï¼›

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Construction and Expression of Vector with aroA-In Gene and Its Transformation in Tobacco

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