Team:Slovenia/Polypeptide manufacturing Idea Approach.html
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+ | <font size="3" color="#009ee0"><b>Polypeptide manufacturing</b></font> | ||
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+ | ==Summary== | ||
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+ | One of the main problems in manufacturing polypeptides is that the isolation and sometimes production method varies from protein to protein, depending on their properties. We prepared the required BioBricks and introduced a procedure that streamlines and unifies manufacturing of polypeptides which results, in principle independently of their sequence, in high yield polypeptide production in bacteria. We demonstrated that peptide production of which in bacteria is difficult due to proteolytic degradation of small unstructured polypeptides, its toxicity to bacteria, such as in antimicrobial peptides and difficult isolation due to small size, can be successfully and in high yield produced as a fusion partner of insoluble ketosteroid isomerase (KSI). Further, acidic cleavage of an Asp-Pro dipeptide between KSI carrier and desired polypeptide is a simple and efficient way for releasing the preferred polypeptide. Since the KSI remains insoluble after cleavage, polypeptide can be easily isolated with HPLC. | ||
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==The idea & Approach== | ==The idea & Approach== | ||
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Revision as of 23:26, 21 October 2009
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Summary
The idea & Approach
Figure 1: Principle of a simple and uniform production of polypeptide biobricks. Polypeptide biobricks are produced as a fusion partner with insoluble ketosteroid isomerase (KSI) in form of inclusion bodies. The linker between KSI and polypeptide biobrick contains acid-labile bond Asp-Pro enabling easy cleavage by acid hydrolysis and separation of polypeptide biobrick from KSI. His-tag may aid in additional initial purification of inclusion bodies or removal of KSI segment in case that the polypeptide is also insoluble under the native conditions and detection of bacterial product by Western blot. |