dc.contributor.author |
Sajitha, S |
|
dc.contributor.author |
Vidhya, J |
|
dc.contributor.author |
Varsha, K |
|
dc.contributor.author |
Binod, P |
|
dc.contributor.author |
Pandey, A |
|
dc.date.accessioned |
2016-06-01T05:39:52Z |
|
dc.date.available |
2016-06-01T05:39:52Z |
|
dc.date.issued |
2015-10-15 |
|
dc.identifier.citation |
Biochemical Engineering Journal 102:14-17 2015 |
en_US |
dc.identifier.uri |
http://hdl.handle.net/123456789/2304 |
|
dc.description.abstract |
l-Asparaginase is an anti-cancer agent which prevents the proliferation of cancerous cells by decreasing
the level of asparagine in the blood. l-asparaginase from Escherichia coli which is encoded by ansB gene is
widely used because of its substrate specificity and less glutaminase activity. Here, we are reporting the
expression studies in yeast which has many added advantages like protein folding and processing. The
expression studies were carried out in a new protein expression system based on the yeast Pichia pastoris
called PichiaPinkTM. ansB gene isolated from E. coli which is coded for asparaginase was cloned into
pPink HC- plasmid and transformed into protease knock out pichia pink strain by electroporation. The
recombinantenzymewasextracellular and showing the activity of 2.5 IU/ml. Itwasthen purified using Ni-
NTA column since the enzyme contains His-tag at the C-terminal end. The new way of expression would
be efficient in making the enzyme humanized by glycosylation patterns which is similar to mammals. |
en_US |
dc.language.iso |
en |
en_US |
dc.publisher |
Elsevier |
en_US |
dc.subject |
Enzyme technology Auxotroph Submerged culture;Recombinant DNA;Asparaginase ;Pichia pink |
en_US |
dc.title |
Cloning and expression of L-Asparaginase from E-coli in Eukaryotic expression system |
en_US |
dc.type |
Article |
en_US |