èŠ‚ç‚¹æ–‡çŒ®

è‹¦èžéº¦ä¸»è¦è¿‡æ•è›‹ç™½Nç«¯åŸºå› ç‰‡æ®µçš„å…‹éš†åŠåºåˆ—åˆ†æž

Cloning and Sequence Analysis of N-terminal Gene of Major Allergenic Protein in Tartary Buckwheat

æŽ¨è CAJä¸‹è½½
PDFä¸‹è½½
ä¸æ”¯æŒè¿…é›·ç‰ä¸‹è½½å·¥å…·ï¼Œè¯·å–æ¶ˆåŠ é€Ÿå·¥å…·åŽä¸‹è½½ã€‚

ã€ä½œè€…ã€‘ èµµå°çï¼› å¼ æ”¿ï¼› æ™¯å·ï¼› æŽçŽ‰è‹±ï¼› çŽ‹è½¬èŠ±ï¼›

ã€Authorã€‘ ZHAO Xiao-zhen,ZHANG Zheng,JING Wei,LI Yu-ying,WANG Zhuan-hua* (Key Laboratory of Chemical Biology and Molecular Engineering, Ministry of Education, Institute of Biotechnology, Shanxi University, Taiyuan 030006, China)

ã€æœºæž„ã€‘ åŒ–å¦ç”Ÿç‰©å¦ä¸Žåˆ†åå·¥ç¨‹æ•™è‚²éƒ¨é‡ç‚¹å®žéªŒå®¤å±±è¥¿å¤§å¦ç”Ÿç‰©æŠ€æœ¯ç ”ç©¶æ‰€ï¼› åŒ–å¦ç”Ÿç‰©å¦ä¸Žåˆ†åå·¥ç¨‹æ•™è‚²éƒ¨é‡ç‚¹å®žéªŒå®¤å±±è¥¿å¤§å¦ç”Ÿç‰©æŠ€æœ¯ç ”ç©¶æ‰€ å±±è¥¿å¤ªåŽŸ030006ï¼› å±±è¥¿å¤ªåŽŸ030006ï¼›

ã€æ‘˜è¦ã€‘ ä¸ºäº†èŽ·å¾—è‹¦èžéº¦ä¸»è¦è¿‡æ•è›‹ç™½å…¨é•¿åŸºå› å¹¶æ·±å…¥å¼€å±•è‹¦èžè¿‡æ•è›‹ç™½çš„ç ”ç©¶,æœ¬å®žéªŒåœ¨å…ˆå‰èŽ·å¾—çš„è‹¦èžéº¦ä¸»è¦è¿‡æ•è›‹ç™½Cç«¯(TBa)åŸºå› åºåˆ—çš„åŸºç¡€ä¸Š,è®¾è®¡ä¸åŒçš„å¼•ç‰©,ä»¥å¼€èŠ±20då·¦å³çš„è‹¦èžéº¦æžœå®žä¸ºææ–™æå–æ€»RNA,å¹¶ä»¥æ¤RNAä¸ºæ¨¡æ¿,é€šè¿‡RT-PCRå’Œ5â€™-RACEç‰æ–¹æ³•,æ‰©å¢ž,å…‹éš†èŽ·å¾—è‹¦èžéº¦ä¸»è¦è¿‡æ•è›‹ç™½Nç«¯(å‘½åä¸ºTBb)cDNAåºåˆ—ã€‚åºåˆ—åˆ†æžç»“æžœè¡¨æ˜Ž,è¯¥åºåˆ—ç”±1005bpç»„æˆ,å¼€æ”¾é˜…è¯»æ¡†ä¸º960bp,å¯ç¼–ç ä¸€ä¸ªç”±320ä¸ªæ°¨åŸºé…¸æ®‹åŸºç»„æˆçš„åŠŸèƒ½è›‹ç™½ã€‚åŒæºæ€§åˆ†æžæ˜¾ç¤º,æ¤æ ¸è‹·é…¸åºåˆ—ä¸Žç”œèžéº¦è¿‡æ•æ€§è´®è—è›‹ç™½åŠè±†çƒç±»è›‹ç™½çš„åŒæºæ€§è¾¾åˆ°90%ã€‚ç”±æ¤æ ¸è‹·é…¸åºåˆ—æŽ¨å¯¼å‡ºçš„æ°¨åŸºé…¸åºåˆ—ä¸Žç”œèžéº¦13Sè´®è—è›‹ç™½æœ‰84%çš„åŒæºæ€§,ä¸Žç”œèžéº¦ä¸»è¦è¿‡æ•è›‹ç™½æœ‰76%çš„åŒæºæ€§ã€‚è‹¦èžéº¦ä¸»è¦è¿‡æ•è›‹ç™½Nç«¯åŸºå› çš„èŽ·å¾—ä¸ºè¯¥è›‹ç™½çš„é‡ç»„è¡¨è¾¾åŠå…¶ç”Ÿç‰©å¦æ´»æ€§ç‰ç ”ç©¶å»ºç«‹äº†å‰æœŸåŸºç¡€ã€‚æ›´å¤š è¿˜åŽŸ

ã€Abstractã€‘ The N-terminal gene of major allergenic protein in tartary buckwheat (named TBb) was amplified from the total RNA of tartary buckwheat using RT-PCR and 5â€™-rapid amplication of cDNA ends (5â€™-RACE) methods. The TBb gene sequence consisted of 1005 nucleotides and a 960bp open reading frame (ORF) which encoded a protein of 320 amino acids residues. Results of homology analysis revealed that the TBb cDNA sequence shared 90% homology with the major allergenic storage protein and legumin-like protein of common buckwheat. The deduced amino acid sequence shared 84% and 76% homology with the legumin-like 13S storage protein and the major allergenic storage protein of common buckwheat respectively. The obtain- ment of the N-terminal gene of major allergenic protein in tartary buckwheat should lay an important foundation for further study of the tartary buckwheat allergen.æ›´å¤š è¿˜åŽŸ