Frederick Ronnie O, Bergeman Lai, Blommel Paul G, Bailey Lucas J, McCoy Jason G, Song Jikui, Meske Louise, Bingman Craig A, Riters Megan, Dillon Nicholas A, Kunert John, Yoon Jung Whan, Lim Ahyoung, Cassidy Michael, Bunge Jason, Aceti David J, Primm John G, Markley John L, Phillips George N, Fox Brian G
The University of Wisconsin Center for Eukaryotic Structural Genomics and Department of Biochemistry, University of Wisconsin, Room 141B, 433 Babcock Drive, Madison, WI 53706, USA.
J Struct Funct Genomics. 2007 Dec;8(4):153-66. doi: 10.1007/s10969-007-9032-5. Epub 2007 Nov 6.
A simple approach that allows cost-effective automated purification of recombinant proteins in levels sufficient for functional characterization or structural studies is described. Studies with four human stem cell proteins, an engineered version of green fluorescent protein, and other proteins are included. The method combines an expression vector (pVP62K) that provides in vivo cleavage of an initial fusion protein, a factorial designed auto-induction medium that improves the performance of small-scale production, and rapid, automated metal affinity purification of His8-tagged proteins. For initial small-scale production screening, single colony transformants were grown overnight in 0.4 ml of auto-induction medium, produced proteins were purified using the Promega Maxwell 16, and purification results were analyzed by Caliper LC90 capillary electrophoresis. The yield of purified [U-15N]-His8-Tcl-1 was 7.5 microg/ml of culture medium, of purified [U-15N]-His8-GFP was 68 microg/ml, and of purified selenomethione-labeled AIA-GFP (His8 removed by treatment with TEV protease) was 172 microg/ml. The yield information obtained from a successful automated purification from 0.4 ml was used to inform the decision to scale-up for a second meso-scale (10-50 ml) cell growth and automated purification. 1H-15N NMR HSQC spectra of His8-Tcl-1 and of His8-GFP prepared from 50 ml cultures showed excellent chemical shift dispersion, consistent with well folded states in solution suitable for structure determination. Moreover, AIA-GFP obtained by proteolytic removal of the His8 tag was subjected to crystallization screening, and yielded crystals under several conditions. Single crystals were subsequently produced and optimized by the hanging drop method. The structure was solved by molecular replacement at a resolution of 1.7 A. This approach provides an efficient way to carry out several key target screening steps that are essential for successful operation of proteomics pipelines with eukaryotic proteins: examination of total expression, determination of proteolysis of fusion tags, quantification of the yield of purified protein, and suitability for structure determination.
本文描述了一种简单的方法,该方法能够以具有成本效益的方式自动纯化重组蛋白,其纯化水平足以用于功能表征或结构研究。文中包含了对四种人类干细胞蛋白、一种工程化绿色荧光蛋白变体以及其他蛋白的研究。该方法结合了一种能在体内切割初始融合蛋白的表达载体(pVP62K)、一种经过析因设计的自诱导培养基(可提高小规模生产的性能)以及对His8标签蛋白的快速自动金属亲和纯化。对于初始小规模生产筛选,将单菌落转化子在0.4 ml自诱导培养基中过夜培养,使用Promega Maxwell 16纯化产生的蛋白,并通过Caliper LC90毛细管电泳分析纯化结果。纯化后的[U-15N]-His8-Tcl-1产量为7.5 μg/ml培养基,[U-15N]-His8-GFP产量为68 μg/ml,经TEV蛋白酶处理去除His8后的纯化硒代蛋氨酸标记的AIA-GFP产量为172 μg/ml。从0.4 ml成功自动纯化获得的产量信息用于指导扩大规模进行第二轮中规模(10 - 50 ml)细胞培养和自动纯化的决策。从50 ml培养物中制备的His8-Tcl-1和His8-GFP的1H-15N NMR HSQC谱显示出优异的化学位移分散性,这与溶液中适合进行结构测定的良好折叠状态一致。此外,通过蛋白酶去除His8标签获得的AIA-GFP进行了结晶筛选,并在多种条件下得到了晶体。随后通过悬滴法制备并优化了单晶。通过分子置换法在1.7 Å的分辨率下解析了结构。这种方法提供了一种有效的方式来执行蛋白质组学流程中成功处理真核蛋白所需的几个关键目标筛选步骤:检查总表达量、确定融合标签的蛋白水解情况、量化纯化蛋白的产量以及评估其是否适合进行结构测定。
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