Targeting Caspase-3 Gene in rCHO Cell Line by CRISPR/Cas9 Editing Tool and Its Effect on Protein Production in Manipulated Cell Line.

IF 1.8 4区 医学 Q3 PHARMACOLOGY & PHARMACY
Amirabbas Rahimi, Morteza Karimipoor, Reza Mahdian, Atefeh Alipour, Sadi Hosseini, Hooman Kaghazian, Abdolrahim Abbasi, Hosein Shahsavarani, Mohammad Ali Shokrgozar
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引用次数: 0

Abstract

Background: Chinese hamster ovary (CHO) cells are the widely used mammalian cell host for biopharmaceutical manufacturing. During cell cultures, CHO cells lose viability mainly from apoptosis. Inhibiting cell death is useful because prolonging cell lifespans can direct to more productive cell culture systems for biotechnology requests.

Objectives: This study exploited a CRISPR/Cas9 technology to generate site-specific gene disruptions in the caspase-3 gene in the apoptosis pathway, which acts as an apoptotic regulator to extend cell viability in the CHO cell line.

Methods: The STRING database was used to identify the key pro-apoptotic genes to be modified by CRISPR/Cas9 system. The guide RNAs targeting the caspase-3 gene were designed, and vectors containing sgRNA and Cas9 were transfected into CHO cells that expressed erythropoietin as a heterologous protein. Indel formation was investigated by DNA sequencing. Caspase-3 expression was quantified by real-time PCR and western blot. The effect of editing the caspase-3 gene on the inhibition of apoptosis was also investigated by induction of apoptosis in manipulated cell lines by oleuropein. Finally, the erythropoietin production in the edited cells was compared to the control cells.

Results: The caspase-3 manipulation significantly prolongation of the cell viability and decreased the caspase-3 expression level of protein in manipulated CHO cells (more than 6-fold, P-value < 0.0001). Manipulated cells displayed higher threshold tolerance to apoptosis compared to the control cells when they were induced by oleuropein. They show a higher IC50 than the control ones (7271 µM/mL Vs. 5741 µM/mL). They also show a higher proliferation rate than the control cells in the presence of an apoptosis inducer (P-value < 0.0001). Furthermore, manipulated cell lines significantly produce more recombinant protein in the presence of 2,000 µM oleuropein compared to the control ones (P-value = 0.0021).

Conclusions: We understood that CRISPR/Cas9 could be effectively applied to suppress the expression of the caspase-3 gene and rescue CHO cells from apoptosis induced by cell stress and metabolites. The CRISPR/Cas9 system-assisted caspase-3 gene ablation can potentially increase erythropoietin yield in CHO cells.

Abstract Image

Abstract Image

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利用CRISPR/Cas9编辑工具靶向rCHO细胞株Caspase-3基因及其对操纵细胞株蛋白生成的影响
背景:中国仓鼠卵巢细胞(CHO)是广泛应用于生物制药生产的哺乳动物细胞宿主。在细胞培养过程中,CHO细胞主要因凋亡而丧失活力。抑制细胞死亡是有用的,因为延长细胞寿命可以为生物技术要求提供更高效的细胞培养系统。目的:本研究利用CRISPR/Cas9技术对凋亡通路中的caspase-3基因进行位点特异性基因破坏,caspase-3基因在CHO细胞系中作为凋亡调节因子延长细胞活力。方法:利用STRING数据库识别CRISPR/Cas9系统修饰的促凋亡关键基因。设计靶向caspase-3基因的引导rna,将含有sgRNA和Cas9的载体转染到以异源蛋白形式表达促红细胞生成素的CHO细胞中。通过DNA测序研究Indel的形成。实时荧光定量PCR和western blot检测Caspase-3的表达。编辑caspase-3基因对细胞凋亡的抑制作用也通过橄榄苦苷诱导细胞凋亡进行了研究。最后,将编辑细胞中的促红细胞生成素的产生与对照细胞进行比较。结果:caspase-3处理可显著延长CHO细胞活力,降低CHO细胞caspase-3蛋白表达水平(p值< 0.0001)。在橄榄苦苷诱导下,与对照细胞相比,处理细胞对凋亡表现出更高的耐受阈值。IC50值高于对照(7271µM/mL Vs. 5741µM/mL)。在存在凋亡诱导剂的情况下,它们的增殖率也高于对照细胞(p值< 0.0001)。此外,与对照组相比,在含有2000µM橄榄苦苷的情况下,处理的细胞株显著产生了更多的重组蛋白(p值= 0.0021)。结论:我们了解CRISPR/Cas9可以有效抑制caspase-3基因的表达,挽救CHO细胞因细胞应激和代谢物诱导的凋亡。CRISPR/Cas9系统辅助caspase-3基因消融可以潜在地增加CHO细胞的促红细胞生成素产量。
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来源期刊
CiteScore
3.40
自引率
6.20%
发文量
52
审稿时长
2 months
期刊介绍: The Iranian Journal of Pharmaceutical Research (IJPR) is a peer-reviewed multi-disciplinary pharmaceutical publication, scheduled to appear quarterly and serve as a means for scientific information exchange in the international pharmaceutical forum. Specific scientific topics of interest to the journal include, but are not limited to: pharmaceutics, industrial pharmacy, pharmacognosy, toxicology, medicinal chemistry, novel analytical methods for drug characterization, computational and modeling approaches to drug design, bio-medical experience, clinical investigation, rational drug prescribing, pharmacoeconomics, biotechnology, nanotechnology, biopharmaceutics and physical pharmacy.
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