Tie Hieng Chiong, Madugula Viswanadh, Lu Lei
School of Biological Sciences, Nanyang Technological University, 60 Nanyang Drive, 637551, Singapore.
School of Biological Sciences, Nanyang Technological University, 60 Nanyang Drive, 637551, Singapore.
Biochem Biophys Res Commun. 2016 Sep 30;478(4):1694-9. doi: 10.1016/j.bbrc.2016.09.005. Epub 2016 Sep 6.
We report here an image-based method to quantify the stoichiometry of diffraction-limited sub-cellular protein complexes in vivo under spinning disk confocal microscopy. A GFP single molecule fluorescence standard was first established by immobilizing His-tagged GFP molecules onto the glass surface via nickel nitrilotriacetic acid functionalized polyethylene glycol. When endogenous nucleoporins were knocked down and replaced by the exogenously expressed and knockdown-resistant GFP-nucleoporins, the stoichiometry of the nucleoporin was estimated by the ratio of its fluorescence intensity to that of the GFP single molecules. Our measured stoichiometry of Nup35, Nup93, Nup133 and Nup88 is 23, 18, 14 and 9 and there are possibly16 copies of Nup107-160 complex per nuclear pore complex.
我们在此报告一种基于图像的方法,用于在旋转盘共聚焦显微镜下对体内衍射极限的亚细胞蛋白质复合物的化学计量进行定量。首先通过将His标签的GFP分子经由次氮基三乙酸镍功能化的聚乙二醇固定在玻璃表面上,建立了GFP单分子荧光标准。当内源性核孔蛋白被敲低并用外源表达且抗敲低的GFP-核孔蛋白替代时,通过其荧光强度与GFP单分子荧光强度的比值来估计核孔蛋白的化学计量。我们测得Nup35、Nup93、Nup133和Nup88的化学计量分别为23、18、14和9,并且每个核孔复合物可能有16个拷贝的Nup107-160复合物。
