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pComb3XSS噬菌体展示质粒

pComb3XSS噬菌体展示质粒

价格: 980

品牌:钦胜生物

供货周期: 现货

货号:QSP0862

规格:2UG

pComb3XSS噬菌体展示质粒

 

基本信息

 

启动子: Lac/lac promoter

质粒大小: 4991bp

质粒标签: C-6×HIS,C-HA

原核抗性: 氨苄青霉素Amp

克隆菌株: 大肠杆菌Stbl3

培养条件: 37℃,有氧,LB

 

质粒简介

        pComb3XSS是一个噬菌体展示质粒。pComb3X is the newest of the pComb vectors. Improvements over pComb3 include increased stability and introduction of an asymmetric SfiI cassette for directional cloning of full Fab, scFv, peptide and other protein for phage display. 6xHis and HA tags allow for purification and detection. An amber stop codon was introduced to turn-off expression of the pIII fusion protein by switching to a non-supressor strain of E. coli allowing production of soluble protein without subcloning. Alternatively, the gene for phage protein pIII can be removed by SpeI/NheI digest. pComb3XSS is recommended for preparation of vector for library cloning. The “SS” refers to the double stuffer, a 1200bp stuffer in the Fab light chain cloning region bounded by SacI and XbaI restriction sites and a 300bp stuffer in Fab heavy chain cloning region bound by XhoI and SpeI restriction sites. Also, the 1600bp double stuffer (both stuffers plus the leader sequence between the Fab light chain and heavy chain cloning regions) can be removed by SfiI digest so that non-Fab genes of interest can be cloned. Also available on Addgene: pComb3XTT and pComb3XLambda are only needed at templates for the construction of chimeric Fab libraries as described in Phage Display: A Laboratory Manual. pComb3XTT can also be used as an Fab expression control. 3rd generation plasmid for phage display on modified geneIII, contains stuffer fragment.

 

质粒图谱

 

扩增流程
         收到产品后,请先根据产品管壁标签来判断产品形式,并在扩增前准确查找该质粒的抗性、感受态和培养温度。
        1、质粒干粉(请务必转化挑单克隆重提后使用)
        ①收到质粒干粉后请先5000rpm离心1min,再加入20μl 无菌水溶解质粒;
        ②2μl质粒加至100μl 感受态中,冰浴30min后,42℃热激60s,不要搅动,再冰浴2min
(从第二步开始均要在超净工作台中无菌操作)

        ③加入500μl无抗的LB液体培养基,180rpm震荡培养45min

        ④10μl100μl复苏液,并分别涂布至目标质粒抗性的LB平板上;
(可使用本平台的平板涂布专用玻璃珠进行涂布,可以比传统涂布方法获得更多转化子)

        ⑤将平板正向培养1h,再倒置37度培养16h。如果要求是30度则培养20h
(如果菌落过多,请将质粒稀释后再转化。如果无菌落,请加入10μl质粒离心全涂转化)

        ⑥挑取单菌落至LB液体培养基中,加入对应抗生素,220rpm震荡培养14h,根据实验需要和质粒提取试剂盒说明书提取质粒。

        2、甘油菌:四区划线后挑单菌落培养,酵母菌需要先液体复苏再四区划线,再挑单菌落液体培养。

        3、穿刺菌:穿刺接种,液体培养后四区划线,再挑单菌落液体培养。

        4、平板:直接挑取单菌落至液体培养基中。
        5、液体质粒:单独提取的液体质粒收到后可直接使用。

 





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