Stable Production of a Tethered Recombinant Eel Luteinizing Hormone Analog with High Potency in CHO DG44 Cells

Author:

Byambaragchaa Munkhzaya1,Park Sei Hyen2,Kim Sang-Gwon2,Shin Min Gyu3,Kim Shin-Kwon3,Hur Sung-Pyo4,Park Myung-Hum12,Kang Myung-Hwa5,Min Kwan-Sik126ORCID

Affiliation:

1. Carbon-Neutral Resources Research Center, Hankyong National University, Anseong 17579, Republic of Korea

2. Graduate School of Animal Biosciences, Hankyong National University, Anseong 17579, Republic of Korea

3. Aquaculture Research Division, National Institute of Fisheries Science, Busan 46083, Republic of Korea

4. Department of Marine Life Science, Jeju National University, Jeju 63243, Republic of Korea

5. Department of Food Science and Nutrition, Hoseo University, Asan 31499, Republic of Korea

6. Division of Animal BioScience, School of Animal Life Convergence Sciences, Institute of Genetic Engineering, Hankyong National University, Anseong 17579, Republic of Korea

Abstract

We produced a recombinant eel luteinizing hormone (rec-eel LH) analog with high potency in Chinese hamster ovary DG44 (CHO DG44) cells. The tethered eel LH mutant (LH-M), which had a linker comprising the equine chorionic gonadotropin (eLH/CG) β-subunit carboxyl-terminal peptide (CTP) region (amino acids 115 to 149), was inserted between the β-subunit and α-subunit of wild-type tethered eel LH (LH-wt). Monoclonal cells transfected with the tethered eel LH-wt and eel LH-M plasmids were isolated from five to nine clones of CHO DG44 cells, respectively. The secreted quantities abruptly increased on day 3, with peak levels of 5000–7500 ng/mL on day 9. The molecular weight of tethered rec-eel LH-wt was 32–36 kDa, while that of tethered rec-eel LH-M increased to approximately 38–44 kDa, indicating the detection of two bands. Treatment with the peptide N-glycanase F decreased the molecular weight by approximately 8 kDa. The oligosaccharides at the eCG β-subunit O-linked glycosylation sites were appropriately modified post-translation. The EC50 value and maximal responsiveness of eel LH-M increased by approximately 2.90- and 1.29-fold, respectively, indicating that the mutant exhibited more potent biological activity than eel LH-wt. Phosphorylated extracellular regulated kinase (pERK1/2) activation resulted in a sharp peak 5 min after agonist treatment, with a rapid decrease thereafter. These results indicate that the new tethered rec-eel LH analog had more potent activity in cAMP response than the tethered eel LH-wt in vitro. Taken together, this new eel LH analog can be produced in large quantities using a stable CHO DG44 cell system.

Funder

National Institute of Fisheries Science

Publisher

MDPI AG

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