èŠ‚ç‚¹æ–‡çŒ®

è—»çº¢è›‹ç™½æ ‡è®°æŠ—é¸¡IgGè§å…‰æŠ—ä½“çš„é«˜æ•ˆåˆ¶å¤‡

Preparation of phycoerythrin-labelled anti-avian-IgG-antibody

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€‘ é¢œä¸–æ•¢ï¼› æœ±ä¸½èï¼› å¼ çŽ‰å¿ ï¼› å‘¨ç™¾æˆï¼› å¼ ç§€ç¾Žï¼›

ã€Authorã€‘ YAN Shi-gan1,3, ZHU Li-ping2, ZHANG Yu-zhong1, ZHOU Bai-cheng1, ZHANG Xiu-mei3(1.State Key Laboratory of Microbial Technology, Shandong University, Jinan 250100, China;2.School of Food and Bioengineering, Shandong Institute of Light Industry, Jinan 250353, China;3.Institute of Animal Husbandry and Veterinary Medicine, Shandong Academy of Agricultural Sciences, Shandong Key Laboratory of Disease Control and Animal Breeding, Jinan 250100, China )

ã€æœºæž„ã€‘ å±±ä¸œå¤§å¦å¾®ç”Ÿç‰©æŠ€æœ¯å›½å®¶é‡ç‚¹å®žéªŒå®¤ï¼› å±±ä¸œçœå†œä¸šç§‘å¦é™¢ç•œç‰§å…½åŒ»ç ”ç©¶æ‰€å±±ä¸œçœåŠ¨ç‰©ç–«ç—…é˜²æŽ§ä¸Žç¹è‚²é‡ç‚¹å®žéªŒå®¤ï¼› å±±ä¸œè½»å·¥ä¸šå¦é™¢é£Ÿå“ä¸Žç”Ÿç‰©å·¥ç¨‹å¦é™¢ï¼›

ã€æ‘˜è¦ã€‘ è—»çº¢è›‹ç™½çš„æ–¯æ‰˜å…‹ä½ç§»å¤§,è§å…‰é‡åäº§çŽ‡é«˜,è§å…‰æ˜Žäº®,æ˜¯ä¸€ç§åº”ç”¨å‰æ™¯å¹¿é˜”çš„è§å…‰æŸ“æ–™ã€‚åˆ¶çº¦è—»çº¢è›‹ç™½åº”ç”¨çš„ä¸»è¦å› ç´ æ˜¯åˆ†ç¦»çº¯åŒ–å›°éš¾åŠå…¶æˆå“å”®ä»·æ˜‚è´µã€‚é€šè¿‡æˆ‘ä»¬å·²ç»å»ºç«‹çš„è—»çº¢è›‹ç™½ä½Žæˆæœ¬é«˜æ•ˆåˆ¶å¤‡å¹³å°,ä½¿å…¶åº”ç”¨äºŽé¢„é˜²å…½åŒ»å¦æ£€æµ‹æˆä¸ºå¯èƒ½ã€‚é¦–æ¬¡é‡‡ç”¨é€‚å®œæ‘©å°”æµ“åº¦çš„äº¤è”å‰‚SPDPå°†è—»çº¢è›‹ç™½ä¸ŽæŠ—é¸¡IgGæŠ—æŠ—ä½“ä»¥æ‘©å°”æ¯”1âˆ¶1é«˜æ•ˆäº¤è”,ç»é«˜æ•ˆæ¶²ç›¸è‰²è°±æ³•çº¯åŒ–åˆ¶å¤‡å‡ºè—»çº¢è›‹ç™½æ ‡è®°çš„æŠ—é¸¡IgGè§å…‰æŠ—æŠ—ä½“ã€‚æœ¬ç ”ç©¶å¯¹åˆ¶å¤‡çš„è§å…‰æŠ—æŠ—ä½“ä»Žè§å…‰ç‰¹æ€§ã€å¸æ”¶å…‰è°±ç‰¹æ€§ã€æŠ—ä½“æ´»æ€§ã€çº¯åº¦åŠç¨³å®šæ€§ç‰æ–¹é¢è¿›è¡Œäº†é‰´å®šã€‚ç»“æžœè¡¨æ˜Ž,è—»çº¢è›‹ç™½æ ‡è®°çš„æŠ—é¸¡IgGè§å…‰æŠ—ä½“ä¸ºç”µæ³³çº¯,è§å…‰æ˜Žäº®,æŠ—ä½“æ´»æ€§é«˜,æ€§è´¨ç¨³å®š,å¯ç”¨äºŽé¸¡ä¼ æŸ“ç—…çš„é—´æŽ¥å…ç–«è§å…‰æ£€æµ‹ã€‚æ›´å¤š è¿˜åŽŸ

ã€Abstractã€‘ Phycoerythrin is an excellent fluorescent dye because of its high fluorescence quantum yield and large stokes shift.However, complicated purification procedure and high price of phycoerythrin hindered its wide application.In this study, an efficient method for preparation of R-phycoerythrin-labelled anti-avian IgG autibody was established using optimum concentration of crosslinker SPDP.The labelled antibody was purified with HPLC and tested for absorption and fluorescence spectra, bioreactivity, and stability.The result showed that the purified labelled antibody had good bioreactivity and stability, which could be widely applied for immunofluorescence detection of avian infectious diseases.æ›´å¤š è¿˜åŽŸ