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Cloning and expression of TagI restriction endonuclease gene using pMAL-c2 vector system in different strains of escherichia coli

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dc.contributor Graduate Program in Chemical Engineering.
dc.contributor.advisor Kırdar, Betül.
dc.contributor.advisor Hortaçsu, Amable.
dc.contributor.author Özkırımlı, Elif.
dc.date.accessioned 2023-03-16T11:08:02Z
dc.date.available 2023-03-16T11:08:02Z
dc.date.issued 1998.
dc.identifier.other CHE 1998 Oz5
dc.identifier.uri http://digitalarchive.boun.edu.tr/handle/123456789/14771
dc.description.abstract The thermostable TaqI restriction endonuclease from Thermus aquaticus was cloned into Escherichia coli for overproduction and single step affinity chromatography purification. The gene was cloned into pMAL-c2 vector, resulting in the cytoplasmic expression of a MBP-TaqI restriction endonuclease fusion protein. In the first part of this study, TaqI restriction endonuclease gene was amplified using Taq DNA polymerase and cloned into E. coli. Although the expected size fusion protein was produced, no endonuclease activity was obtained. Growth condition manipulations and expression in different strains did not result in the production of an active enzyme. Subsequent sequencing of the gene indicated a mutation at position 410 that might abolish activity. In the second part, cloning was repeated after amplification of the gene with Pfu DNA polymerase which has proofreading activity. A colony coding for a protein with the expected size and activity was identified. Upon optimization of induction time, higher tiled was obtained when the culture was induced at an absorbance of 0.9. Expression in three different strains of E. coli, indicated total recovery was higher in TB1 cells at 300,000 Units/liter of culture volume as compared to 100,000 Units/liter in XL1-Blue cells and 150,000 Units/liter in ER2508 cells.
dc.format.extent 30 cm.
dc.publisher Thesis (M.S.) - Bogazici University.Institute for Graduate Studies in Science and Engineering, 1998.
dc.relation Includes appendices.
dc.relation Includes appendices.
dc.subject.lcsh Escherichia coli.
dc.subject.lcsh Proteins -- Biotechnology.
dc.subject.lcsh DNA polymerases.
dc.title Cloning and expression of TagI restriction endonuclease gene using pMAL-c2 vector system in different strains of escherichia coli
dc.format.pages xii, 114 leaves;


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