| نویسندگان | Hassan Rassouli, Ali Sayadmanesh, Siamak Rezaeiani, Zahra Ghezelayagh, Mohammad Reza Gharaati, Yaser Tahamtani |
|---|---|
| نشریه | Cell journal |
| عنوان لاتين مجله | Cell journal |
| نوع مقاله | Original Research |
| تاریخ انتشار | 2020/7/1 |
| رتبه نشریه | ISI |
| نوع نشریه | چاپی |
| کشور محل چاپ | ایران |
چکیده مقاله
Abstract
Objective: Growth factors are key elements of embryonic stem cell (ESC) research. Cell line development in eukaryotes
is a time-consuming procedure which usually takes 12-18 months. Here, we report an easy and fast method with which
production of Chinese hamster ovary (CHO) cells that express and secrete recombinant Activin A, as a major growth
factor in endo/mesoderm differentiation of embryonic stem cells is achieved within 3-4 weeks.
Materials and Methods: In this experimental study, we cloned human Activin A into the pDONR/Zeo gateway entry
vector using the BP reaction. Activin A was subcloned next into the pLIX_403 and pLenti6.3/TO/V5-DEST destination
vectors by the LR reaction. The result was the production of constructs with which 293T cells were finally transfected
for virus production. CHO cells were transduced using viral particles to produce a cell line that secretes the His6- Activin
A fusion protein.
Results: We developed a quick protocol which saves up to 3-4 weeks of time for producing recombinant proteins in
CHO cells. The recombinant cell line produced 90 mg/L of functional Activin A measured in human ESC line Royan H5
(RH5), during in vitro differentiation into meso-endoderm and definitive endoderm.
Conclusion: Our results showed no significant differences in functionality between commercial Activin A and the one
produced using our novel protocol. This approach can be easily used for producing recombinant proteins in CHO.