A1 Refereed original research article in a scientific journal
Enhanced cell density cultivation and rapid expression-screening of recombinant Pichia pastoris clones in microscale
Authors: Neha Kaushik, Urpo Lamminmäki, Navin Khanna, Gaurav Batra
Publisher: Nature Research
Publication year: 2020
Journal:Scientific Reports
Journal name in sourceScientific Reports
Volume: 10
Issue: 1
Number of pages: 11
ISSN: 2045-2322
DOI: https://doi.org/10.1038/s41598-020-63995-5
Self-archived copy’s web address: https://research.utu.fi/converis/portal/detail/Publication/48042915
Cultivation of yeast Pichia pastoris in the microtiter plate, for
 optimisation of culture conditions, and expression screening of 
transformants has gained significance in recent years. However, in the 
microtiter plate, it has been challenging to attain cell densities 
similar to well-aerated shake-flask culture, due to the poor mixing 
resulting in oxygen limitation. To solve this problem, we investigated 
the influence of multiple cultivation parameters on P. pastoris 
cell growth, including the architecture of 96-deepwell plate (96-DWP), 
shaking throw diameter, shaking frequency, culture volume/well, and 
media composition. In the optimised conditions, a cell density of OD600
 ~50 (dry cell weight ~13 g/L) with >99% cell viability was achieved 
in the casamino acids supplemented buffered-minimal-media in 300 to 
1000 μl culture volume/well. We have devised a simplified method 
for coating of the culture supernatant on the polystyrene surface for 
immunoassay. Clones for secretory expression of envelope domain III of 
dengue virus serotype-1 under the control of inducible and constitutive 
promoter were screened using the developed method. Described microscale 
cultivation strategy can be used for rapid high-throughput screening of P. pastoris
 clones, media optimization, and high-throughput recombinant protein 
production. The knowledge gained through this work may also be applied, 
to other suspension cultures, with some modifications.
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