动物营养学报
動物營養學報
동물영양학보
ACTA ZOONUTRIMENTA SINICA
2014年
11期
3349-3355
,共7页
陈小玲%王欢%黄志清%周波%贾刚%刘光芒%赵华
陳小玲%王歡%黃誌清%週波%賈剛%劉光芒%趙華
진소령%왕환%황지청%주파%가강%류광망%조화
猪PID1%原核表达%纯化%质谱鉴定%多克隆抗体
豬PID1%原覈錶達%純化%質譜鑒定%多剋隆抗體
저PID1%원핵표체%순화%질보감정%다극륭항체
porcine PID1%prokaryotic expression%purification%mass spectrum identification%polyclonal anti-body
本文旨在通过原核表达获得猪磷酸酪氨酸互作结构域1( pPID1)重组蛋白,并制备pPID1多克隆抗体。将pPID1基因插入pET28a(+),构建重组pET28a(+)-pPID1大肠杆菌表达质粒,然后将重组质粒pET28a(+)-pPID1转化到大肠杆菌BL21感受态细胞中,获得的重组子以不同异丙基硫代-β-D-半乳糖苷( IPTG)浓度、温度和时间诱导,确定pPID1融合蛋白表达的最适条件。将表达产物经镍离子-亚氨基二乙酸( Ni2+-IDA)亲和层析纯化后进行基质辅助激光解析电离飞行时间质谱( MALDI-TOF-MSMS)鉴定。同时,将纯化获得的pPID1融合蛋白免疫SD大鼠,制备pPID1多克隆抗体,并检测抗体效价。结果表明:pPID1融合蛋白表达的最佳条件为30℃以0.1 mmol/L IPTG 诱导4 h;纯化的融合蛋白经 MALDI-TOF-MSMS 鉴定为pPID1;特异性的pPID1多克隆抗体成功制备,抗体效价为1∶20480。本试验成功制备了高纯度的重组pPID1及其多克隆抗体。
本文旨在通過原覈錶達穫得豬燐痠酪氨痠互作結構域1( pPID1)重組蛋白,併製備pPID1多剋隆抗體。將pPID1基因插入pET28a(+),構建重組pET28a(+)-pPID1大腸桿菌錶達質粒,然後將重組質粒pET28a(+)-pPID1轉化到大腸桿菌BL21感受態細胞中,穫得的重組子以不同異丙基硫代-β-D-半乳糖苷( IPTG)濃度、溫度和時間誘導,確定pPID1融閤蛋白錶達的最適條件。將錶達產物經鎳離子-亞氨基二乙痠( Ni2+-IDA)親和層析純化後進行基質輔助激光解析電離飛行時間質譜( MALDI-TOF-MSMS)鑒定。同時,將純化穫得的pPID1融閤蛋白免疫SD大鼠,製備pPID1多剋隆抗體,併檢測抗體效價。結果錶明:pPID1融閤蛋白錶達的最佳條件為30℃以0.1 mmol/L IPTG 誘導4 h;純化的融閤蛋白經 MALDI-TOF-MSMS 鑒定為pPID1;特異性的pPID1多剋隆抗體成功製備,抗體效價為1∶20480。本試驗成功製備瞭高純度的重組pPID1及其多剋隆抗體。
본문지재통과원핵표체획득저린산락안산호작결구역1( pPID1)중조단백,병제비pPID1다극륭항체。장pPID1기인삽입pET28a(+),구건중조pET28a(+)-pPID1대장간균표체질립,연후장중조질립pET28a(+)-pPID1전화도대장간균BL21감수태세포중,획득적중조자이불동이병기류대-β-D-반유당감( IPTG)농도、온도화시간유도,학정pPID1융합단백표체적최괄조건。장표체산물경얼리자-아안기이을산( Ni2+-IDA)친화층석순화후진행기질보조격광해석전리비행시간질보( MALDI-TOF-MSMS)감정。동시,장순화획득적pPID1융합단백면역SD대서,제비pPID1다극륭항체,병검측항체효개。결과표명:pPID1융합단백표체적최가조건위30℃이0.1 mmol/L IPTG 유도4 h;순화적융합단백경 MALDI-TOF-MSMS 감정위pPID1;특이성적pPID1다극륭항체성공제비,항체효개위1∶20480。본시험성공제비료고순도적중조pPID1급기다극륭항체。
The aim of this experiment was to construct recombinant protein of porcine phosphotyrosine interac-tion domain containing 1 ( pPID1 ) by prokaryotic expression system and prepare polyclonal antibody against the recombinant pPID1. pPID1 gene was cloned into the prokaryotic expression vector pET28a(+). The re-combinant expression plasmid pET28a(+)-pPID1 was constructed and then transformed into Escherichia coli ( E. coli) BL21 to express pPID1. The recombinant pPID1 was induced by the addition of isopropylβ-D-thio-galactopyranoside ( IPTG) . To optimize the expression of recombinant pPID1, IPTG concentration, tempera-ture and time after induction by IPTG were varied. The recombinant protein was purified by Ni2+-iminodiacetic acid( IDA) affinity chromatography and was identified using matrix-assisted laser desorption/ionization time of flight mass spectrometry ( MALDI-TOF-MSMS) . To prepare polyclonal antibody against pPID1, the purified fusion protein was used to immunize Sprague Dawley ( SD) rats and the antibody titer was determined. The re-sults showed that pPID1 was expressed at a high level when the recombinant E. coli BL21 was induced with 0.1 mmo/L IPTG for 4 h at 30℃;MALDI-TOF-MSMS analysis confirmed that the purified fusion protein was pPID1;the specific polyclonal antibody against pPID1 with the titer of 1 ∶ 20 480 was obtained. The highly pu-rified recombinant pPID1 protein and its polyclonal antibody were successfully prepared in the present study.
