Kumar Niraj, Gammell Patrick, Meleady Paula, Henry Michael, Clynes Martin
National Institute for Cellular Biotechnology, Dublin City University, Glasnevin, Dublin 9, Ireland.
BMC Biotechnol. 2008 Apr 22;8:42. doi: 10.1186/1472-6750-8-42.
To ensure maximal productivity of recombinant proteins (rP) during production culture it is typical to encourage an initial phase of rapid cell proliferation to achieve high biomass followed by a stationary phase where cellular energies are directed towards production of rP. During many such biphasic cultures, the initial phase of rapid cell growth at 37 degrees C is followed by a growth arrest phase induced through reduction of the culture temperature. Low temperature induced growth arrest is associated with many positive phenotypes including increased productivity, sustained viability and an extended production phase, although the mechanisms regulating these phenotypes during mild hypothermia are poorly understood.
In this study differential protein expression in suspension CHO-K1 cells was investigated following a reduction of the culture temperature from 37 degrees C to 31 degrees C in comparison to standard batch culture maintained at 37 degrees C using 2D-DIGE (Fluorescence 2-D Difference Gel Electrophoresis) and mass spectrometry (MS). There is only limited proteomic analysis of suspension-grown CHO cells describing a direct comparison of temperature shifted versus non-temperature shifted cultures using 2D-DIGE. This investigation has enabled the identification of temperature-dependent as well as temperature-independent proteomic changes. 201 proteins were observed as differentially expressed following temperature shift, of which 118 were up regulated. Of the 53 proteins identified by MALDI-ToF MS, 23 were specifically differentially expressed upon reduction of the culture temperature and were found related to a variety of cellular functions such as regulation of growth (HNRPC), cap-independent translation (EIF4A), apoptosis (importin-alpha), the cytoskeleton (vimentin) and glycoprotein quality control (alpha glucosidase 2).
These results indicate the extent of the temperature response in CHO-K1 cells and suggest a number of key regulatory proteins and pathways that are involved in modulating the response of cells to mild hypothermia. Regulation of these identified proteins and pathways could be useful for future approaches to engineer CHO cells for improved recombinant protein production.
为确保生产培养过程中重组蛋白(rP)的最大产量,通常会促进细胞快速增殖的初始阶段以实现高生物量,随后进入稳定期,此时细胞能量导向rP的生产。在许多这样的双相培养中,37℃下细胞快速生长的初始阶段之后是通过降低培养温度诱导的生长停滞阶段。低温诱导的生长停滞与许多积极表型相关,包括提高产量、维持活力和延长生产阶段,尽管在轻度低温期间调节这些表型的机制尚不清楚。
在本研究中,与使用二维差异凝胶电泳(2D-DIGE)和质谱(MS)维持在37℃的标准分批培养相比,研究了悬浮CHO-K1细胞在培养温度从37℃降至31℃后的差异蛋白表达。关于悬浮培养的CHO细胞的蛋白质组学分析有限,使用2D-DIGE描述了温度变化与未温度变化培养的直接比较。这项研究能够识别温度依赖性和非温度依赖性的蛋白质组学变化。温度变化后观察到201种蛋白质差异表达,其中118种上调。在通过基质辅助激光解吸电离飞行时间质谱(MALDI-ToF MS)鉴定的53种蛋白质中,23种在培养温度降低时特异性差异表达,并且发现与多种细胞功能相关,如生长调节(HNRPC)、非帽依赖性翻译(EIF4A)、细胞凋亡(输入蛋白-α)、细胞骨架(波形蛋白)和糖蛋白质量控制(α葡萄糖苷酶2)。
这些结果表明CHO-K1细胞中温度反应的程度,并提示了一些参与调节细胞对轻度低温反应的关键调节蛋白和途径。对这些已鉴定的蛋白质和途径的调节可能有助于未来改造CHO细胞以提高重组蛋白产量的方法。
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