Effect of Different Additive Factors on the Growth and Antibody Secretion of Hybridoma Cells
ZHANG Song-Yu, ZENG Xin-Yi*, ZHU Yuan-Tao*, LI Zhi-Yuan, SU Jun**, LI Qiu-Yan**
College of Biological Sciences/State Key Laboratory of Animal Biotech Breeding/National Demonstration Center for Experimental Education of Life Science, China Agricultural University, Beijing 100193, China
Abstract:The hybridoma cell technique is a crucial method for monoclonal antibody production. Monoclonal antibody-producing hybridoma cells against Porcine epidemic diarrhea virus (PEDV) have been prepared in this research group. In this study, the hybridoma cell culture system was optimized to improve the efficiency of antibody secretion from hybridoma cells by adding different concentrations of additive factors, including glutamine (0~10 mmol/L), antimicrobial peptides (0~20 μg/mL), peptides (0~20 ng/mL), human epidermal growth factor (hEGF) (0~20 ng/mL), basic fibroblast growth factor (bFGF)(0~20 ng/mL), and vitamin C (VitC)(0~20 ng/mL). These factors were introduced into the hybridoma cell culture system to investigate their impact on the growth and antibody secretion of hybridoma cells by plotting growth curves and using enzyme-linked immunosorbent assay (ELISA), respectively. The results showed that the peak of cell density was reached on the 5th day when glutamine and antimicrobial peptides were added, and the maximum cell density was achieved at the addition concentration of 6 mmol/L glutamine and 10 μg/mL antimicrobial peptides. The peak of cell density was reached on the 4th day when hEGF, bFGF and VitC were added, and the maximum cell density was achieved at the addition concentration of 10 ng/mL hEGF, 20 ng/mL bFGF and 20 ng/mL VitC. The results of antibody titer detection showed that the highest antibody titer (1∶8000) was obtained in the glutamine addition group at a concentration of 6 mmol/L, the highest antibody titer (1∶16000) was obtained in the antimicrobial peptide addition group at a concentration of 10 μg/mL, the highest antibody titer (1∶16000) was obtained in the hEGF and bFGF addition groups at concentrations of 5 and 10 ng/mL, respectively, and the highest antibody titer (1∶8000) was obtained in the VitC addition group at a concentration of 10 ng/mL. In conclusion, the growth and antibody production capabilities of hybridoma cells have been effectively enhanced through the modification of medium components. This study establishes a solid groundwork for the formulation of specialized hybridoma cell culture media aimed at production purposes.
张松雨, 曾馨仪, 朱源涛, 李志远, 苏俊, 李秋艳. 不同添加因子对杂交瘤细胞生长和抗体分泌的影响[J]. 农业生物技术学报, 2025, 33(2): 379-385.
ZHANG Song-Yu, ZENG Xin-Yi, ZHU Yuan-Tao, LI Zhi-Yuan, SU Jun, LI Qiu-Yan. Effect of Different Additive Factors on the Growth and Antibody Secretion of Hybridoma Cells. 农业生物技术学报, 2025, 33(2): 379-385.
[1] 郭芳睿, 秦俊红, 李彦霖, 等. 2017. 细胞无血清培养现状概述[J]. 生物技术通讯, 28(6): 865-870. (Guo F R, Qin J H, Li Y L, et al.2017. Overview of current status of serum-free cell culture[J]. Letters in Biotechnology, 28(6): 865-870.) [2] 商瑜, 张启明, 李悦, 等. 2015. 动物细胞无血清培养基的发展和应用[J]. 陕西师范大学学报(自然科学版), 43(4): 68-72. (Shang Y, Zhang Q M, Li Y, et al.2015. Progress on serum-free media of zooblast[J]. Journal of Shaanxi Normal University (Natural Science Edition), 43(4): 68-72.) [3] 王朋朋, 黄书林, 张云科, 等. 2021. 哺乳动物细胞无血清全悬浮培养技术研究进展[J]. 中国畜牧兽医, 48(03): 839-845. (Wang P P, Huang S L, Zhang Y K, et al.2021. Research progress on serum-free suspension culture of mammalian cells[J]. China Animal Husbandry & Veterinary Medicine, 48(03): 839-845.) [4] 武荣飞, 杨溢, 王鹏志, 等. 2022. 单克隆抗体制备技术最新研究进展[J]. 中国预防兽医学报, 44(3): 333-337, 343. (Wu R F, Yang Y, Wang P Z, et al.2022. Recent advances in monoclonal antibody production technology[J]. Chinese Journal of Preventive Veterinary Medicine, 44(3): 333-337, 343.) [5] 张淑香, 李东晓, 朱明龙, 等. 2008. 谷氨酰胺限制对杂交瘤细胞生长、代谢和单抗生产的影响[J]. 高校化学工程学报, 22(1): 77-82. (Zhang S X, Li D X, Zhu M L, et al.2008. Effect of glutamine limitation on growth, metabolism and mAb production of hybridoma cells[J]. Journal of Chemical Engineering of Chinese Universities, 22(1): 77-82.) [6] Bushell M E, Bell S L, Scott M F, et al.1993. A 3-phase pattern in growth, monoclonal-antibody production, and metabolite exchange in a hybridoma bioreactor culture[J]. Biotechnology and Bioengineering, 42(1): 133-139. [7] Dandulakis G, Herr J C, Kirwan D J.1997. Effect of growth factors and antigen on hybridoma cell culture dynamics[J]. Biotechnology and Bioengineering, 54(4): 357-364. [8] Hosios A M, Hecht V C, Danai L V, et al.2016. Amino acids rather than glucose account for the majority of cell mass in proliferating mammalian cells[J]. Developmental Cell, 36(5): 540-549. [9] John B, Gertrude B, Lia H C, et al.2017. Best practices in cell culture: An overview[J]. In vitro Cellular and Devel‐opmental Biology-Animal, 53(9): 669-672. [10] Jost M, Kari C, Rodeck U.2000. The hEGF receptor - an essential regulator of multiple epidermal functions[J]. European Journal of Dermatology, 10(7): 505-510. [11] Jung K, Saif L J.2015. Porcine epidemic diarrhea virus infection: Etiology, epidemiology, pathogenesis and immunoprophylaxis[J]. Veterinary Journal, 204(2): 134-143. [12] Kohler G, Milstein C.1975. Continuous cultures of fused cells secreting antibody of predefined specificity[J]. Nature, 256(5517): 495-497. [13] Kouakanou L, Xu Y, Peters C, et al.2020. Vitamin C promotes the proliferation and effector functions of human γδT cells[J]. Cellular & Molecular Immunology, 17(5): 462-473. [14] Li L, Mi L, Feng Q, et al.2005. Increasing the culture efficiency of hybridoma cells by the use of integrated metabolic control of glucose and glutamine at low levels[J]. Biotechnology and Applied Biochemistry, 42(Pt 1): 73-80. [15] Liu Y, Chi L, Feng L, et al.2012. Effects of graded levels of dietary vitamin C on the growth, digestive capacity and intestinal microflora of juvenile Jian carp[J]. Progress in Veterinary Medicine, 33(8):41-46. [16] Moraes J Z, Hamaguchi B, Braggion C, et al.2021. Hybridoma technology: Is it still useful?[J]. Current Research in Immunology, 3(2): 32-40. [17] Nelson P N, Reynolds G M, Waldron E E, et al.2000. Monoclonal antibodies[J]. Journal of Clinical Pathology-Molecular Pathology, 53(3): 111-117. [18] Newland M, Greenfield P F, Reid S.1990. Hybridoma growth limitations - the roles of energy-metabolism and ammonia production[J]. Cytotechnology, 3(3): 215-229. [19] Parray H A, Shukla S, Samal S, et al.2020. Hybridoma technology a versatile method for isolation of monoclonal antibodies, its applicability across species, limitations, advancement and future perspectives[J]. International Immunopharmacology, 85: 106639. [20] Pendse G J, Bailey J E.1990. Effects of growth-factors on cell-proliferation and monoclonal-antibody production of batch hybridoma cultures[J]. Biotechnology Letters, 12(7): 487-492. [21] Schneider M, Marison I W, Vonstockar U.1996. The importance of ammonia in mammalian cell culture[J]. Journal of Biotechnology, 46(3): 161-185. [22] Song D, Park B.2012. Porcine epidemic diarrhoea virus: A comprehensive review of molecular epidemiology, diagnosis, and vaccines[J]. Virus Genes, 44(2): 167-175. [23] Xu X, Sun H, Cui H, et al.2023. Immunomodulatory effect of antimicrobial peptide hi-3 from Hermetia illucens l.On raw264.7 cells[J]. Journal of Environmental Entomology, 45(2): 464-472. [24] Yang T, Li J, Jia Q, et al.2021. Antimicrobial peptide 17BIPHE2 inhibits the proliferation of lung cancer cells in vitro and in vivo by regulating the ERK signaling pathway[J]. Oncology Letters. 22(1): 501. [25] Zhan S, Li J, Yang T, et al.2019. Antimicrobial peptide merecidin induces apoptosis in human lung adenocarcinoma cell line A549[J]. Basic & Clinical Medicine, 39(4): 473-477.
