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首页> 美国卫生研究院文献>BMC Microbiology >Correction to: Interaction of the heterotrimeric G protein alpha subunit SSG-1 of Sporothrix schenckii with proteins related to stress response and fungal pathogenicity using a yeast two-hybrid assay
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Correction to: Interaction of the heterotrimeric G protein alpha subunit SSG-1 of Sporothrix schenckii with proteins related to stress response and fungal pathogenicity using a yeast two-hybrid assay

机译:校正至:酵母双杂交法检测申氏孢子菌的异三聚体G蛋白α亚基SSG-1与与应激反应和真菌致病性有关的蛋白质的相互作用

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Co-immunoprecipitation and Western Blot analyses of SSG-1 interacting proteins. corresponds to the results of the Co-IP of SSG-1 and SsSOD, corresponds to the results of the Co-IP of SSG-1 and SsNramp, corresponds to the results of the Co-IP of SSG-1 and SsSit and corresponds to the results of the Co-IP of SSG-1 and SsGAPDH. Whole cell free extracts of cells expressing the complete c-myc tagged SSG-1 coding sequence fused to the GAL4 activation domain (prey protein) and the HA tagged protein fragment fused to the GAL4 DNA binding domain (bait protein) were co-immunoprecipitated as described in Methods. The coimmunoprecipitated proteins were separated using 10% SDS polyacrylamide electrophoresis under non-reducing conditions and transferred to nitrocellulose. Lane 1: Nitrocellulose strips were probed with anti-cMyc antibody as the primary antibody and anti-mouse IgG as the secondary antibody that recognizes both the heavy and light chain of the anti-cMyc (The two high molecular weight bands present belong to the anti-cMyc antibody used for precipitation). Lane 2: Negative controls where no primary antibody was added and probed with the secondary antibody anti-mouse IgG that recognizes both the heavy and light chain of the anti-cMyc antibody. Lane 3: Nitrocellulose strips were probed with anti-HA antibody as the primary antibody and anti-rabbit IgG as the secondary antibody that recognizes both the heavy and light chain of the anti-HA. Lane 4: Negative controls where no primary antibody was added and probed with the secondary antibody anti-rabbit IgG that recognizes both the heavy and light chain of the anti-HA antibody. Pre-stained molecular weight markers were included in outside lanes of the gel. Exposure times to detect the interacting proteins SSSOD using anti-cMyc antibodies and antiHA antibodies were 3.1 s and 9.1 s, respectively. To detect the other binding partners SSNRAMP, SSSIT, and SSGAPDH using anti-cMyc antibody and anti-HA antibody were 1 s for each one
机译:SSG-1相互作用蛋白的免疫共沉淀和蛋白质印迹分析。对应于SSG-1和SsSOD的Co-IP的结果,对应于SSG-1和SsNramp的Co-IP的结果,对应于SSG-1和SsSit的Co-IP的结果,并且对应于SSG-1和SsGAPDH的Co-IP的结果。将表达完整c-myc标签的SSG-1编码序列融合到GAL4激活域(猎物蛋白)和HA标签蛋白片段融合到GAL4 DNA结合域(诱饵蛋白)的细胞的全细胞无提取物,进行免疫共沉淀。在方法中描述。在非还原条件下,使用10%SDS聚丙烯酰胺电泳分离共免疫沉淀的蛋白质,并将其转移到硝酸纤维素膜上。泳道1:以识别抗cMyc的重链和轻链的抗cMyc抗体作为一抗,抗小鼠IgG作为二抗探测硝酸纤维素条(存在的两个高分子量带属于抗-cMyc抗体用于沉淀)。泳道2:阴性对照,其中未添加一抗并用识别抗cMyc抗体的重链和轻链的二抗抗小鼠IgG进行探测。泳道3:用识别抗HA的重链和轻链的抗HA抗体作为第一抗体和抗兔IgG作为第二抗体来探测硝酸纤维素条。泳道4:阴性对照,其中不添加一抗,并用识别抗HA抗体的重链和轻链的二抗抗兔IgG进行探测。预先染色的分子量标记包括在凝胶的外部泳道中。使用抗cMyc抗体和抗HA抗体检测相互作用蛋白SSSOD的暴露时间分别为3.1µs和9.1µs。为了检测其他结合伴侣,使用抗cMyc抗体和抗HA抗体的SSNRAMP,SSSIT和SSGAPDH分别为1µs

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