Two Simple Methods for Optimizing the Production of "Difficult-to-Express" GnRH-DFF40 Chimeric Protein

Purpose: GnRH-DFF40 (gonadotropin releasing hormone - DNA fragmentation factor 40) is a humanized recombinant immunotoxin and serves as a prospective candidate for targeted therapy of gonadotropin releasing hormone receptor (GnRHR) overexpressing malignancies. However, its production in Escherichia...

Descripción completa

Detalles Bibliográficos
Autores principales: Barazesh, Mahdi, Mostafavipour, Zohreh, Kavousipour, Soudabeh, Mohammadi, Shiva, Mokarram, Pooneh
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Tabriz University of Medical Sciences 2019
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6773931/
https://www.ncbi.nlm.nih.gov/pubmed/31592077
http://dx.doi.org/10.15171/apb.2019.050
_version_ 1783455989061648384
author Barazesh, Mahdi
Mostafavipour, Zohreh
Kavousipour, Soudabeh
Mohammadi, Shiva
Mokarram, Pooneh
author_facet Barazesh, Mahdi
Mostafavipour, Zohreh
Kavousipour, Soudabeh
Mohammadi, Shiva
Mokarram, Pooneh
author_sort Barazesh, Mahdi
collection PubMed
description Purpose: GnRH-DFF40 (gonadotropin releasing hormone - DNA fragmentation factor 40) is a humanized recombinant immunotoxin and serves as a prospective candidate for targeted therapy of gonadotropin releasing hormone receptor (GnRHR) overexpressing malignancies. However, its production in Escherichia coli in a soluble and functional form still remains a challenge. Here we introduce two successful and reproducible conditions for production and purification of “difficult-to-express” GnRH-DFF40 protein. Methods: A synthetic codon optimized GnRH-DFF40 fusion gene was cloned in pET28a plasmid. Two methods including high cell density IPTG induction (HCDI) and autoinduction method (AIM) with a focus on obtaining high cell density have been investigated to enhance the protein production in (E. coli). Moreover, to obtain higher protein production several factors in the AIM method including carbon sources, incubation time and temperature, plasmid stability and double colony selection, were optimized. Results: Remarkable amounts of soluble GnRH-DFF40 protein were achieved by both methods. Cell density and protein yields in AIM was about 1.5 fold higher than that what obtained using HCDI. Initial screening showed that 25ºC is better to achieve higher protein production in both methods. pH alterations in AIM were maintained in a more constant level at 25ºC and 37ºC temperatures without any detrimental effects on cell growth during protein production phase up to 21 hours after incubation. Plasmid stability during growth and expression induction phase was maintained at a high level of 98% and 96% for AIM and HCDI methods, respectively. After parameter optimization and double colony selection in AIM, a very high yield of recombinant protein was achieved (528.3 mg/L). Conclusion: With the optimization of these high cell density expression methods, reproducible manifold enhancement of soluble protein yields can be achieved for “difficult-to-express” GnRH-DFF40 compared to conventional expression methods.
format Online
Article
Text
id pubmed-6773931
institution National Center for Biotechnology Information
language English
publishDate 2019
publisher Tabriz University of Medical Sciences
record_format MEDLINE/PubMed
spelling pubmed-67739312019-10-07 Two Simple Methods for Optimizing the Production of "Difficult-to-Express" GnRH-DFF40 Chimeric Protein Barazesh, Mahdi Mostafavipour, Zohreh Kavousipour, Soudabeh Mohammadi, Shiva Mokarram, Pooneh Adv Pharm Bull Research Article Purpose: GnRH-DFF40 (gonadotropin releasing hormone - DNA fragmentation factor 40) is a humanized recombinant immunotoxin and serves as a prospective candidate for targeted therapy of gonadotropin releasing hormone receptor (GnRHR) overexpressing malignancies. However, its production in Escherichia coli in a soluble and functional form still remains a challenge. Here we introduce two successful and reproducible conditions for production and purification of “difficult-to-express” GnRH-DFF40 protein. Methods: A synthetic codon optimized GnRH-DFF40 fusion gene was cloned in pET28a plasmid. Two methods including high cell density IPTG induction (HCDI) and autoinduction method (AIM) with a focus on obtaining high cell density have been investigated to enhance the protein production in (E. coli). Moreover, to obtain higher protein production several factors in the AIM method including carbon sources, incubation time and temperature, plasmid stability and double colony selection, were optimized. Results: Remarkable amounts of soluble GnRH-DFF40 protein were achieved by both methods. Cell density and protein yields in AIM was about 1.5 fold higher than that what obtained using HCDI. Initial screening showed that 25ºC is better to achieve higher protein production in both methods. pH alterations in AIM were maintained in a more constant level at 25ºC and 37ºC temperatures without any detrimental effects on cell growth during protein production phase up to 21 hours after incubation. Plasmid stability during growth and expression induction phase was maintained at a high level of 98% and 96% for AIM and HCDI methods, respectively. After parameter optimization and double colony selection in AIM, a very high yield of recombinant protein was achieved (528.3 mg/L). Conclusion: With the optimization of these high cell density expression methods, reproducible manifold enhancement of soluble protein yields can be achieved for “difficult-to-express” GnRH-DFF40 compared to conventional expression methods. Tabriz University of Medical Sciences 2019-08 2019-08-01 /pmc/articles/PMC6773931/ /pubmed/31592077 http://dx.doi.org/10.15171/apb.2019.050 Text en © 2019 The Author (s) http://creativecommons.org/licenses/by/4.0/ This is an Open Access article distributed under the terms of the Creative Commons Attribution (CC BY), which permits unrestricted use, distribution, and reproduction in any medium, as long as the original authors and source are cited. No permission is required from the authors or the publishers.
spellingShingle Research Article
Barazesh, Mahdi
Mostafavipour, Zohreh
Kavousipour, Soudabeh
Mohammadi, Shiva
Mokarram, Pooneh
Two Simple Methods for Optimizing the Production of "Difficult-to-Express" GnRH-DFF40 Chimeric Protein
title Two Simple Methods for Optimizing the Production of "Difficult-to-Express" GnRH-DFF40 Chimeric Protein
title_full Two Simple Methods for Optimizing the Production of "Difficult-to-Express" GnRH-DFF40 Chimeric Protein
title_fullStr Two Simple Methods for Optimizing the Production of "Difficult-to-Express" GnRH-DFF40 Chimeric Protein
title_full_unstemmed Two Simple Methods for Optimizing the Production of "Difficult-to-Express" GnRH-DFF40 Chimeric Protein
title_short Two Simple Methods for Optimizing the Production of "Difficult-to-Express" GnRH-DFF40 Chimeric Protein
title_sort two simple methods for optimizing the production of "difficult-to-express" gnrh-dff40 chimeric protein
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6773931/
https://www.ncbi.nlm.nih.gov/pubmed/31592077
http://dx.doi.org/10.15171/apb.2019.050
work_keys_str_mv AT barazeshmahdi twosimplemethodsforoptimizingtheproductionofdifficulttoexpressgnrhdff40chimericprotein
AT mostafavipourzohreh twosimplemethodsforoptimizingtheproductionofdifficulttoexpressgnrhdff40chimericprotein
AT kavousipoursoudabeh twosimplemethodsforoptimizingtheproductionofdifficulttoexpressgnrhdff40chimericprotein
AT mohammadishiva twosimplemethodsforoptimizingtheproductionofdifficulttoexpressgnrhdff40chimericprotein
AT mokarrampooneh twosimplemethodsforoptimizingtheproductionofdifficulttoexpressgnrhdff40chimericprotein

Ejemplares similares