SPI “sandwich”: Combined <scp>SUMO‐Peptide‐Intein</scp> expression system and isolation procedure for improved stability and yield of peptides

Lamer, Tess; Belkum, Marco J. van; Wijewardane, Anjalee; Chiorean, Sorina; Martin‐Visscher, Leah A.; Vederas, John C.

doi:10.1002/pro.4316

Cited by 15 publications

(19 citation statements)

References 34 publications

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“…That the entire system (containing Bsa BI blunt restriction enzyme site) can be transferred to any vector, we confirmed by the construction of additional pQE_Ek expression vector (Figure 1). Based on the latest results in the development of new improved expression vectors, we can conclude that the improvement of expression vectors will most likely go in the direction of reducing the toxicity of expressed AMPs (sandwich tag vector construction) and those contributing to AMP modification to increase stability and functionality (Lamer et al, 2022; Zhu et al, 2021). The improvements we have presented in this study can be combined with other improvements (most are compatible) in the construction of new expression vectors with multiple tags (sandwich tag) and with enzymatic modifications and processing.…”

Section: Discussionmentioning

confidence: 99%

Redesigned pMAL expression vector for easy and fast purification of active native antimicrobial peptides

Gardijan

Miljković

Obradović

et al. 2022

Journal of Applied Microbiology

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The aim of this study was to construct the improved pMAL expression vector to increase the efficacy of purification of small native peptides and their clear-cut separation from MBP tag. The modifications we introduced can be applied to many expression vectors. Methods and Results:To improve the pMAL expression vector, we introduced the His 6 tag and the enterokinase cleavage site (Ek) downstream from the MBP tag and Xa cleavage site on the original vector. For cloning of a desired peptide DNA, the enterokinase site contains a unique BsaBI restriction site adjacent to the original multi-cloning site. This redesigned pMAL vector was optimized for the purification of cytoplasmic (pMALc5HisEk) and periplasmic (pMALp5HisEk) peptides. The purification of native and active peptide (P) was obtained following two-step affinity chromatography. In the first step, the entire MBP-His 6 -Ek-P fusion protein is purified using the Ni-NTA agarose column. This fusion protein was cleaved with active His 6 tagged enterokinase.In the second step, the further purification was performed by column containing the mixture of amylose and Ni-NTA agarose resins. This removes both the MBP-His 6 and His 6 -enterokinase leaving pure native protein in solution. These new vectors and the two-step purification protocol were successfully applied in purification of active native small antimicrobial peptides (AMPs), lactococcin A and human βdefensin. Conclusions: We constructed the improved pMAL expression vectors and established the pipeline and optimal conditions for their use in efficient purification of large amounts of active native small peptides.Significance and Impact of the Study: Choice of expression vector impacts on the efficiency of expression and purification of desired proteins. The idea of redesigning pMAL vector was driven by the need for rapid purification of larger amounts of active native AMPs. This newly improved pMAL vector, the cloning strategy, expression conditions and two-step purification protocol represent a unique simple approach which can be applied in every laboratory. K E Y W O R D Scomplete removal of tags and proteinase, His 6 -enterokinase cleavage site, improved pMAL and pQE vectors, native antimicrobial peptides, two-step chromatography

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Section: Discussionmentioning

confidence: 99%

Redesigned pMAL expression vector for easy and fast purification of active native antimicrobial peptides

Gardijan

Miljković

Obradović

et al. 2022

Journal of Applied Microbiology

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“…MALDI‐TOF MS of SUMO‐peptide fusion protein and cleaved intein after overnight incubation of an SPI fusion protein in 100 mM DTT. Example mass spectrum for purification of the bacteriocin peptide faerocin MK (Lamer et al., 2022). Figure adapted from Lamer et al.…”

Section: Commentarymentioning

confidence: 99%

“…kDa = Molecular weight standards in kilodaltons. Example results for purification of the bacteriocin peptide leucocin A (Lamer et al., 2022). Lanes: MW, PageRuler Prestained Protein Ladder; 1, SUMO‐peptide fusion protein before addition of SUMO protease; 2, after incubation of SUMO‐peptide fusion protein with SUMO protease for 2 hr; 3, flowthrough from the final Ni‐NTA column; 4, wash (20 mM imidazole) final Ni‐NTA column; 5, elution (500 mM imidazole) of final Ni‐NTA column.…”

Section: Commentarymentioning

confidence: 99%

“…Figures were created with Biorender.com. Figures 3, 4, 5, 6, and 8 were adapted from Lamer et al (2022) with permission.…”

Section: Acknowledgmentsmentioning

confidence: 99%

“…The small ubiquitin‐like modifier (SUMO) is a common fusion tag choice for peptides, as cleavage is completed by addition of a highly specific SUMO protease that leaves no extra residues behind on the peptide of interest (Butt, Edavettal, Hall, & Mattern, 2005). However, isolation of peptides as SUMO fusion proteins can be complicated by degradation of the fusion protein during expression in E. coli (Lamer et al., 2022). This can be a major problem if a large amount of peptide is needed for downstream applications, as the final yield of purified peptide can be quite low.…”

Section: Introductionmentioning

confidence: 99%

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Methods for Recombinant Production and Purification of Peptides as SUMO‐Peptide‐Intein Fusion Proteins to Protect from Degradation

2022

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Heterologous expression in Escherichia coli is a commonly used method to produce ribosomally synthesized peptides for further study. This generally requires expression of the target protein with an affinity fusion tag, followed by isolation of the fusion protein from a cellular lysate by affinity purification, and finally by removal of the fusion tag and purification of the desired peptide. Sometimes, however, fusion proteins may be degraded during recombinant expression in E. coli. We recently reported an expression system that sandwiches the target peptide between an N‐terminal small ubiquitin‐like modifier (SUMO) protein and a C‐terminal intein. This SUMO‐peptide‐intein (SPI) fusion protein protects the central peptide from degradation and can lead to improved peptide yield after purification. In this report, we detail the cloning, expression, and isolation procedures for the SPI fusion system, with comments on conditions that can be optimized for different peptides to obtain maximal yield for each construct. © 2022 Wiley Periodicals LLC. Basic Protocol 1: Cloning to construct SPI gene Basic Protocol 2: Expression of SPI fusion proteins in E. coli BL21(DE3) Support Protocol: Optimization of expression and induction conditions Basic Protocol 3: Isolation and purification of SPI fusion proteins with a chitin column Alternate Protocol: Isolation and purification of SPI fusion proteins without chitin

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Encouraging Solution to the Problem of Synthesizing Protein α‐Thioester

Liu,

Gao,

Zhao

et al. 2024

Chin. J. Chem.

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Comprehensive SummaryExpressed protein ligation (EPL) provides a powerful tool to access large‐size proteins with precise structures. Existing methods for constructing the critical protein thioester for EPL have predominantly relied on the recombinant intein fusion expressed in Escherichia coli (E. coli). Despite its powerful applications, the expression of thioester derived from eukaryotic protein in E. coli inherently suffers from its limited solubility, the inactivity of intein, premature hydrolysis and low yields. To overcome these obstacles, we present herein the facile one‐flask synthesis of inaccessible protein α‐thioester via a SUMO‐protein‐intein (SPI) sandwich model. The utility of SUMO enhances the protein fusion yield and solubility, prevents premature hydrolysis and simplifies the purification process. The inaccessible protein thioester with internal Cys residues can be readily produced and is compatible with the EPL‐desulfurization protocol used to prepare complex proteins, which is otherwise difficult to obtain using traditional methods. Its utility has been highlighted through the synthesis of human granulocyte colony‐stimulating factor (G‐CSF).

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SPI “sandwich”: Combined SUMO‐Peptide‐Intein expression system and isolation procedure for improved stability and yield of peptides

Cited by 15 publications

References 34 publications

Redesigned pMAL expression vector for easy and fast purification of active native antimicrobial peptides

Redesigned pMAL expression vector for easy and fast purification of active native antimicrobial peptides

Methods for Recombinant Production and Purification of Peptides as SUMO‐Peptide‐Intein Fusion Proteins to Protect from Degradation

Encouraging Solution to the Problem of Synthesizing Protein α‐Thioester

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