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优化缩减规模的串联亲和纯化以鉴定核心蛋白复合物

Optimisation of Downscaled Tandem Affinity Purifications to Identify Core Protein Complexes.

作者信息

Haura Eric B, Sacco Roberto, Li Jiannong, Müller André C, Grebien Florian, Superti-Furga Giulio, Bennett Keiryn L

机构信息

Department of Thoracic Oncology Program, H. Lee Moffitt Cancer Center and Research Institute, Tampa, Florida, USA.

出版信息

J Integr OMICS. 2012 May;2(1):55-68. doi: 10.5584/jiomics.v2i1.81.

Abstract

In this study we show that via stable, retroviral-expression of tagged EGFR del (L747-S752 deletion mutant) in the PC9 lung cancer cell line and stable doxycycline-inducible expression of tagged Grb2 using a Flp-mediated recombination HEK293 cell system, the SH-TAP can be downscaled to 5 to 12.5 mg total protein input (equivalent to 0.5 - 1 × 15 cm culture plate or 4 - 8 × 10 cells). The major constituents of the EGFR del complex (USB3B, GRB2, ERRFI, HSP7C, GRP78, HSP71) and the Grb2 complex (ARHG5, SOS1, ARG35, CBL, CBLB, PTPRA, SOS2, DYN2, WIPF2, IRS4) were identified. Adjustment of the quantity of digested protein injected into the mass spectrometer reveals that optimisation is required as high quantities of material led to a decrease in protein sequence coverage and the loss of some interacting proteins. This investigation should aid other researchers in performing tandem affinity purifications in general, and in particular, from low quantities of input material.

摘要

在本研究中,我们表明,通过在PC9肺癌细胞系中稳定地逆转录病毒表达带标签的EGFR del(L747 - S752缺失突变体),以及使用Flp介导的重组HEK293细胞系统稳定地强力霉素诱导表达带标签的Grb2,SH - TAP可以将总蛋白输入量缩减至5至12.5毫克(相当于0.5 - 1个15厘米培养板或4 - 8×10个细胞)。鉴定了EGFR del复合物(USB3B、GRB2、ERRFI、HSP7C、GRP78、HSP71)和Grb2复合物(ARHG5、SOS1、ARG35、CBL、CBLB、PTPRA、SOS2、DYN2、WIPF2、IRS4)的主要成分。调整注入质谱仪的消化蛋白量表明,由于大量材料会导致蛋白质序列覆盖率降低和一些相互作用蛋白的丢失,因此需要进行优化。这项研究总体上应有助于其他研究人员进行串联亲和纯化,特别是从少量输入材料中进行纯化。

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