High-yield production and purification of the fusion pH-responsive peptide GST-pHLIP in Escherichia coli BL21

IF 0.7 Q4 BIOCHEMISTRY & MOLECULAR BIOLOGY AIMS Molecular Science Pub Date : 2022-01-01 DOI:10.3934/molsci.2022008
Oscar Cienfuegos-Jiménez, Abril Morales-Hernández, Olivia A. Robles‐Rodríguez, Sergio Bustos-Montes, Kevin A. Bañuelos-Alduncin, Aurora R. Cortés-Castillo, Hugo D. Barreto-Hurtado, Luis Carrete-Salgado, I. Marino-Martínez
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Abstract

The pH Low Insertion Peptide (pHLIP) has versatile applications in several diseases due to its differential behavior at slightly different pH values. pHLIP is an unstructured and peripheral membrane-associated peptide at neutral pH and an α-helical transmembrane peptide at acidic values. Similar to what happened to insulin and growth hormone, pHLIP´s expanding applications require high-yield production to further scale-up its usefulness. To date, synthesis of the pHLIP has not been reported in a prokaryotic platform, mainly relying on solid-phase synthesis. Bacterial production arises as an option for high-amount peptide generation and larger pHLIP fusion protein-synthesis; however, cell-based pH-responsive peptide production could be challenging due to intracellular peptide interactions or degradation due to unstructured conformations. An Escherichia coli (E. coli)-BL21 cell culture was induced with Isopropyl ß-D-1-thiogalactopyranoside (IPTG) in order to produce a Glutathione S-transferase-pHLIP (GST-pHLIP) fusion construct. Purification was done with Glutathione (GSH)-decorated magnetic beads using 4 ml of the induced cell culture. The production was quantified with Bradford reagent and characterized with SDS-PAGE and Western blot, contrasting Bradford results with densitometry analysis to obtain production approximate absolute values. A purified approximate total yield of ~26 µg with an apparent GSH-bead saturation and a total production of ~82 µg was obtained. Our Western Blot assay confirmed the presence of the GST-pHLIP construct in all the IPTG-induced fractions. Conclusion: A high-yield pHLIP production irrespective of its membrane affinity in acidic environments or its unstructured nature was achieved. Our study could be useful to scale up pHLIP synthesis for future applications.
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大肠杆菌BL21融合ph响应肽gst - phillip的高产制备与纯化
pH低插入肽(pHLIP)由于其在轻微不同的pH值下的不同行为,在几种疾病中具有广泛的应用。philip是中性pH下的非结构化外周膜相关肽,酸性pH下是α-螺旋跨膜肽。与胰岛素和生长激素类似,pHLIP的应用范围不断扩大,需要高产量的产品来进一步扩大其用途。迄今为止,pHLIP的合成尚未在原核平台上报道,主要依赖于固相合成。细菌生产出现作为一种选择,以产生大量的肽和更大的philips融合蛋白合成;然而,由于细胞内肽相互作用或非结构化构象导致的降解,基于细胞的ph响应肽生产可能具有挑战性。用异丙基ß- d -1-硫代半乳糖苷(IPTG)诱导大肠杆菌(E. coli)-BL21细胞培养,产生谷胱甘肽s -转移酶- phillip (gst - phillip)融合构建体。用4ml诱导细胞培养物用谷胱甘肽(GSH)修饰的磁珠进行纯化。用Bradford试剂定量,SDS-PAGE和Western blot对产量进行表征,将Bradford结果与密度分析进行对比,以获得产量的近似绝对值。纯化后的总产率约为~26µg, GSH-bead明显饱和,总产量约为~82µg。我们的Western Blot检测证实在所有iptg诱导的部分中都存在gst - phillip构建体。结论:无论其在酸性环境中的膜亲和性或非结构化性质如何,均可获得高产率的pHLIP。我们的研究可能有助于扩大philips合成的规模,以用于未来的应用。
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来源期刊
AIMS Molecular Science
AIMS Molecular Science BIOCHEMISTRY & MOLECULAR BIOLOGY-
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4
审稿时长
5 weeks
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