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Titlebook: High-Throughput Protein Production and Purification; Methods and Protocol Renaud Vincentelli Book 2019Latest edition Springer Science+Busin

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A High-Throughput Automated Protein Folding Systemn acceptable yield. Generally this requires screening a matrix of buffers and stabilizers to find an appropriate solution. Herein, we describe an automated and quantitative method to identify optimal in vitro protein folding parameters with a high rate of success.
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Parallelized Microscale Expression of Soluble scFv For this screening procedure, a highly parallelized approach to produce soluble antibody fragments in microtiter plates is essential. In this chapter, we give the protocol for the parallelized microscale production of scFvs for the screening procedure or further assays.
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High-Throughput Isolation of Soluble Protein Domains Using a Bipartite Split-GFP Complementation Sysagging fragment (GFP β-strand 11, or GFP11). The assay is performed in . cells and in cell extracts. A selection step insures the protein fragments are in frame and contain no stop codons, while an inverse PCR is used to enrich protein fragment libraries containing a specific target sequence.
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1064-3745 expertsThis book compiles key protocols instrumental to the study of high-throughput protein production and purification which have been refined and simplified over the years and are now ready to be transferred to any laboratory. Beginning with a section covering general procedures for high-through
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Hot CoFi Blot: A High-Throughput Colony-Based Screen for Identifying More Thermally Stable Protein Vstability—the Hot CoFi blot. We share how to create the random mutagenesis library, how to perform the Hot CoFi blot, and how to identify more thermally stable clones. We use the Tobacco Etch Virus protease as a target to exemplify the procedure.
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