Your search keyword '"Myc-tag"' showing total 513 results

1. In vitro evolution of myc-tag antibodies: in-depth specificity and affinity analysis of Myc1-9E10 and Hyper-Myc.

Author

Russo, Giulio, Unkauf, Tobias, Meier, Doris, Wenzel, Esther Veronika, Langreder, Nora, Schneider, Kai-Thomas, Wiesner, Rebecca, Bischoff, Ralf, Stadler, Volker, and Dübel, Stefan

Subjects

*MONOCLONAL antibodies, *ANTIBODY specificity, *IMMUNOGLOBULINS, *MYC proteins

Abstract

Bacterial supernatant containing monoclonal scFv antibodies was mixed 1:2 with 2% MPBS-T and incubated in the antigen coated plates for 1.5 h at RT followed by three washing steps in PBS-T. Thanks to their C-terminal HIS tag, bound scFv antibodies were detected with mouse anti-hexa-HIS-tag DIA-900 antibody (Dianova, Hamburg, Germany) and goat anti-mouse secondary antibody conjugated to horseradish peroxidase (HRP) (A0168, Sigma). Graph: Figure 2: Epitope mapping studies on peptide array.(A) Hyper-Myc and Myc1-9E10 monoclonal antibodies minimal epitope recognition as determined by PEPperMAP® Epitope Mapping laser printed peptide arrays. Myc1-9E10 (red) or Hyper-Myc (blue) top 1299 peptide hits on PEPperCHIP® Human Epitome Microarray (29,127 human peptides).A fluorescence signal of 2000 is considered in the range of 10% of the signal generated by antibody incubation on myc-epitope peptide. Keywords: epitope mapping; hypermyc; myc-tag; peptide microarrays; phage display; recombinant antibody EN epitope mapping hypermyc myc-tag peptide microarrays phage display recombinant antibody 479 494 16 04/12/22 20220401 NES 220401 Introduction Epitope tags allow for generic detection of transgenic proteins Reverse genetics approaches using gene overexpression, dominant negative, and transgene expression I in vitro i and I in vivo i , opened new ways to assess wild type and mutant gene functions. [Extracted from the article]

Published

2022

2. Detection and purification of backbone-cyclized proteins using a bacterially expressed anti-myc-tag single chain antibody.

Author

Chauhan, Sushma, Hou, Chen Yuan, Jung, Sang Taek, and Kang, Taek Jin

Subjects

*IMMUNOGLOBULINS, *RECOMBINANT proteins, *BACTERIAL antibodies, *ESCHERICHIA coli, *MOLECULAR chaperones

Abstract

A myc-tag and of which recognition by an antibody 9E10 has long been used for the detection and purification of recombinant proteins. We have previously expanded the application of the tag to the specific detection and purification of backbone-cyclized proteins. Here we sought a more practical way to using the 9E10 antibody by expressing its single chain antibody (scAb) form in Escherichia coli . The combined use of a strong T7 promoter and auto-induction strategy rather than early to mid-log induction of a Lac promoter resulted in the soluble over-expression of 9E10 scAb. However, the co-expression of a chaperone, Skp, was absolutely necessary for the activity even when the protein was expressed in a soluble manner. We could purify about 4 mg of 9E10 scAb from 1 l of culture, and the resulting scAb could be used to detect and purify the backbone-cyclized protein as the parental full-length 9E10. Moreover, the immunoaffinity resin prepared using 9E10 scAb could be regenerated several times after the elution of bound proteins using an acid, which added more value to the ready preparation of the active antibody in bacteria. [ABSTRACT FROM AUTHOR]

Published

2017

3. Analysis of the c-Myc tag presence in the CAR’s antigen-recognition domain structural stability, through molecular dynamics simulation

Author

Ana Lima, Natália Fernandes Frota, Alice Queiroz, and Marcos Roberto Lourenzoni

Subjects

Physics, Molecular dynamics, Structural stability, Computational biology, Antigen recognition, Domain (software engineering), Myc-tag

Published

2021

4. The Polymorphic PolyQ Tail Protein of the Mediator Complex, Med15, Regulates the Variable Response to Diverse Stresses

Author

Michael C. Ayers, Nassif C, Amaury Pupo, Ser Sl, and Gallagher Jeg

Subjects

0301 basic medicine, Mediator, 010501 environmental sciences, yeast, 01 natural sciences, lcsh:Chemistry, polyQ, stress, MCHM, protein chaperone, Gene Expression Regulation, Fungal, Gene expression, lcsh:QH301-705.5, Spectroscopy, 2. Zero hunger, Mediator Complex, biology, General transcription factor, Protein Stability, inorganic phosphate, Myc tag, General Medicine, Computer Science Applications, Cell biology, Snf1, Med15, Gene isoform, Saccharomyces cerevisiae Proteins, intrinsically disordered regions, Saccharomyces cerevisiae, Protein Serine-Threonine Kinases, Catalysis, Article, master variator, Inorganic Chemistry, 03 medical and health sciences, Cyclohexanes, Stress, Physiological, transcription factors, hydrotrope, Physical and Theoretical Chemistry, Molecular Biology, Transcription factor, Gene, 0105 earth and related environmental sciences, Organic Chemistry, HSP40 Heat-Shock Proteins, 030104 developmental biology, lcsh:Biology (General), lcsh:QD1-999, Chaperone (protein), Mutation, biology.protein, Peptides, Myc-tag

Abstract

The Mediator is composed of multiple subunits conserved from yeast to humans and plays a central role in transcription. The tail components are not required for basal transcription but are required for responses to different stresses. While some stresses are familiar, such as heat, desiccation, and starvation, others are exotic, yet yeast can elicit a successful stress response. 4-Methylcyclohexane methanol (MCHM) is a hydrotrope that induces growth arrest in yeast. We found that a naturally occurring variation in the Med15 allele, a component of the Mediator tail, altered the stress response to many chemicals in addition to MCHM. Med15 contains two polyglutamine repeats (polyQ) of variable lengths that change the gene expression of diverse pathways. The Med15 protein existed in multiple isoforms and its stability was dependent on Ydj1, a protein chaperone. The protein level of Med15 with longer polyQ tracts was lower and turned over faster than the allele with shorter polyQ repeats. MCHM sensitivity via variation of Med15 was regulated by Snf1 in a Myc-tag-dependent manner. Tagging Med15 with Myc altered its function in response to stress. Genetic variation in transcriptional regulators magnified genetic differences in response to environmental changes. These polymorphic control genes were master variators.

Published

2020

5. The Myc tag monoclonal antibody 9E10 displays highly variable epitope recognition dependent on neighboring sequence context

Author

Stefan Schüchner, Christian Behm, Egon Ogris, and Ingrid Mudrak

Subjects

0303 health sciences, biology, medicine.drug_class, Context (language use), Cell Biology, Monoclonal antibody, Biochemistry, Fusion protein, Molecular biology, Epitope, 03 medical and health sciences, 0302 clinical medicine, Polyclonal antibodies, medicine, biology.protein, Peptide microarray, Antibody, Molecular Biology, 030217 neurology & neurosurgery, 030304 developmental biology, Myc-tag

Abstract

Epitope tags are short, linear antibody recognition sequences that enable detection of tagged fusion proteins by antibodies. Epitope tag position and neighboring sequences potentially affect its recognition by antibodies, and such context-dependent differences in tag binding may have a wide-ranging effect on data interpretation. We tested by Western blotting six antibodies that recognize the c-Myc epitope tag, including monoclonal antibodies 9E10, 4A6, 9B11, and 71D10 and polyclonal antibodies 9106 and A-14. All displayed context-dependent differences in their ability to detect N- or C-terminal Myc-tagged proteins. In particular, clone 9E10, the most cited Myc-tag antibody, displayed high context-dependent detection variability, whereas others, notably 4A6 and 9B11, showed much less context sensitivity in their detection of Myc-tagged proteins. The very high context sensitivity of 9E10 was further substantiated by peptide microarray analyses. We conclude that recently developed, purpose-made monoclonal antibodies specific for Myc have much more uniform reactivity in diverse assays and are much less context sensitive than is the legacy antibody 9E10.

Published

2020

6. AF166 and AI179 antibodies recognize a Myc-tagged recombinant protein by immunofluorescence

Author

Lima, Wanessa Cristina

Subjects

biology, medicine.diagnostic_test, General Medicine, biology.organism_classification, Immunofluorescence, Molecular biology, law.invention, HeLa, law, biology.protein, medicine, Recombinant DNA, Antibody, ddc:612, Myc-tag

Abstract

AF166 and AI179 antibodies against the Myc tag recognize a Myc-tagged human TAC protein by immunofluorescence in paraformaldehyde-fixed HeLa cells; AF372, AF373 and AI831 do not.

Published

2020

7. Anti-c-Myc Tag (9E10) Affinity Gel Protocol v2

Author

Sam Li

Subjects

Chemistry, Molecular biology, Myc-tag

Abstract

Catalog Number: 658502 Storage Temperature: 2°C-8°C Product Description: Anti-c-Myc Tag (9E10) Affinity Gel consists of anti-c-myc monoclonal antibody (clone 9E10), covalently immobilized onto 6% high density glyoxal agarose beads. The affinity resin can be used in affinity purifying and immunoprecipitation of c-Myc-tagged fusion protein. Binding Specificity: Mouse monoclonal antibody 9E10 recognizes the c-myc epitope N-EQKLSEEDL-C and is purified through Protein G chromatography. The antibody conjugated affinity resin can bind to epitope at N-terminal, C-terminal, and internal locations of a fusion protein. The binding capacity is greater than 0.5mg per ml of c-myc agarose resin. Reagent: Anti-c-Myc Agarose Affinity Gel is supplied as a 50% suspension in phosphate-buffered saline, pH 7.2, containing 0.09% sodium azide. Precautions and Disclaimer: This product is for research use only. Please consult the Material Safety Data Sheet for information regarding hazards and safe handling practices. Storage/Stability: Anti-c-Myc Agarose Affinity Gel should be stored between 2°C and 8°C for maximum stability. The unopened product is stable for one year when stored as indicated. After use, the resin should be regenerated and stored in TBS or PBS buffer (pH 7.2) containing 0.09% sodium azide.

Published

2019

8. Detection and purification of backbone-cyclized proteins using a bacterially expressed anti-myc-tag single chain antibody

Author

Sushma Chauhan, Taek Jin Kang, Chen Yuan Hou, and Sang Taek Jung

Subjects

0301 basic medicine, Recombinant Fusion Proteins, Green Fluorescent Proteins, Biophysics, lac operon, Single chain, Protein Engineering, medicine.disease_cause, Biochemistry, law.invention, Proto-Oncogene Proteins c-myc, 03 medical and health sciences, law, Escherichia coli, medicine, Molecular Biology, biology, Escherichia coli Proteins, Cell Biology, biology.organism_classification, Molecular biology, DNA-Binding Proteins, 030104 developmental biology, Cyclization, Chaperone (protein), biology.protein, Recombinant DNA, Antibody, Bacteria, Molecular Chaperones, Single-Chain Antibodies, Myc-tag

Abstract

A myc-tag and of which recognition by an antibody 9E10 has long been used for the detection and purification of recombinant proteins. We have previously expanded the application of the tag to the specific detection and purification of backbone-cyclized proteins. Here we sought a more practical way to using the 9E10 antibody by expressing its single chain antibody (scAb) form in Escherichia coli. The combined use of a strong T7 promoter and auto-induction strategy rather than early to mid-log induction of a Lac promoter resulted in the soluble over-expression of 9E10 scAb. However, the co-expression of a chaperone, Skp, was absolutely necessary for the activity even when the protein was expressed in a soluble manner. We could purify about 4 mg of 9E10 scAb from 1 l of culture, and the resulting scAb could be used to detect and purify the backbone-cyclized protein as the parental full-length 9E10. Moreover, the immunoaffinity resin prepared using 9E10 scAb could be regenerated several times after the elution of bound proteins using an acid, which added more value to the ready preparation of the active antibody in bacteria.

Published

2017

9. Generation of Nanobodies against SlyD and development of tools to eliminate this bacterial contaminant from recombinant proteins

Author

Serge Muyldermans, Francisco Morales-Yánez, Cécile Vincke, Changxiao Liu, Ema Romão, Carlos Gutierrez, Yaozhong Hu, Didier Vertommen, Faculty of Sciences and Bioengineering Sciences, Cellular and Molecular Immunology, and Department of Bio-engineering Sciences

Subjects

0301 basic medicine, Recombinant protein, Camelus, Immunoprecipitation, Size-exclusion chromatography, Isomerase, Immunodominance, Biology, law.invention, 03 medical and health sciences, SlyD, law, Escherichia coli, Animals, Panning (camera), chemistry.chemical_classification, Chromatography, Escherichia coli Proteins, Peptidylprolyl Isomerase, Single-Domain Antibodies, SEC, Recombinant Proteins, BL21 E.coli expression, Amino acid, 030104 developmental biology, chemistry, Biochemistry, Nanobody, Recombinant DNA, IMAC, Biotechnology, Myc-tag

Abstract

The gene for a protein domain, derived from a tumor marker, fused to His tag codons and under control of a T7 promotor was expressed in E. coli strain BL21 (DE3). The recombinant protein was purified from cell lysates through immobilized metal affinity chromatography and size-exclusion chromatography. A contaminating bacterial protein was consistently co-purified, even using stringent washing solutions containing 50 or 100 mM imidazole. Immunization of a dromedary with this contaminated protein preparation, and the subsequent generation and panning of the immune Nanobody library yielded several Nanobodies of which 2/3 were directed against the bacterial contaminant, reflecting the immunodominance of this protein to steer the dromedary immune response. Affinity adsorption of this contaminant using one of our specific Nanobodies followed by mass spectrometry identified the bacterial contaminant as FKBP-type peptidyl-prolyl cis-trans isomerase (SlyD) from E. coli. This SlyD protein contains in its C-terminal region 14 histidines in a stretch of 31 amino acids, which explains its co-purification on Ni-NTA resin. This protein is most likely present to varying extents in all recombinant protein preparations after immobilized metal affinity chromatography. Using our SlyD-specific Nb 5 we generated an immune-complex that could be removed either by immunocapturing or by size exclusion chromatography. Both methods allow us to prepare a recombinant protein sample where the SlyD contaminant was quantitatively eliminated.

Published

2017

10. Immuno-affinity purification of 2B8-tagged proteins

Author

Man-Ho Cho, Hyerin Choi, Tae-Lim Kim, and Seong-Hee Bhoo

Subjects

0301 basic medicine, Linear epitope, medicine.drug_class, Chemistry, Organic Chemistry, Protein tag, Monoclonal antibody, Molecular biology, General Biochemistry, Genetics and Molecular Biology, Epitope, 03 medical and health sciences, 030104 developmental biology, Affinity chromatography, Biochemistry, FLAG-tag, medicine, Peptide sequence, Myc-tag

Abstract

Detection, purification and characterization of proteins are essential procedures in the field of biochemistry. Epitope tag systems are commonly used to characterize unknown proteins. The Deinococcus radiodurans bacterial phytochrome (DrBphP) protein has been used as an antigen to generate anti-DrBphP mouse monoclonal antibodies and to identify their specific epitopes. Among these antibodies, the 2B8 monoclonal antibody recognizes an epitope of 9 amino acids (RDPLPFFPP). The 2B8 epitope does not match the amino acid sequence for any known protein. On Western blot analysis, the 2B8 antibody showed strong and highly specific interactions with the 2B8 epitope. These results suggest that the 2B8 epitope-antibody is a useful epitope tag system for protein characterization. In addition, we generated a modified epitope (RDPLPAFPP) via point mutation in a previous study. This modified epitope showed significantly increased reactivity with the 2B8 antibody. In this study, we developed a protein purification system using the 2B8 epitope tag and antibody. 2B8 antibodies were bound to protein G-agarose beads as affinity ligands. Recombinant DrBphP proteins were then exposed to 2B8 antibody-bound protein G-agarose beads. Bound DrBphP proteins were then eluted by competition with the original or modified 2B8 epitope peptides. DrBphP proteins were successfully purified via an affinity chromatography system using a 2B8 original peptide and even better purified using the 2B8 modified peptide. These findings indicate that the 2B8 epitope tag system is a better tool for protein detection and purification.

Published

2017

11. Use of a protein engineering strategy to overcome limitations in the production of 'Difficult to Express' recombinant proteins

Author

Hirra Hussain, W. Mark Abbott, Robert G. Roth, David I Fisher, and Alan J. Dickson

Subjects

0301 basic medicine, Low protein, Protein family, Bioengineering, Protein engineering, Biology, Applied Microbiology and Biotechnology, Protein subcellular localization prediction, Cell biology, 03 medical and health sciences, 030104 developmental biology, Biochemistry, biology.protein, Furin, Peptide sequence, Secretory pathway, Biotechnology, Myc-tag

Abstract

Certain recombinant proteins are deemed "difficult to express" in mammalian expression systems requiring significant cell and/or process engineering to abrogate expression bottlenecks. With increasing demand for the production of recombinant proteins in mammalian cells, low protein yields can have significant consequences for industrial processes. To investigate the molecular mechanisms that restrict expression of recombinant proteins, naturally secreted model proteins were analyzed from the tissue inhibitors of metalloproteinase (TIMP) protein family. In particular, TIMP-2 and TIMP-3 were subjected to detailed study. TIMP proteins share significant sequence homology (∼50% identity and ∼70% similarity in amino acid sequence). However, they show marked differences in secretion in mammalian expression systems despite this extensive sequence homology. Using these two proteins as models, this study characterized the molecular mechanisms responsible for poor recombinant protein production. Our results reveal that both TIMP-2 and TIMP-3 are detectable at mRNA and protein level within the cell but only TIMP-2 is secreted effectively into the extracellular medium. Analysis of protein localization and the nature of intracellular protein suggest TIMP-3 is severely limited in its post-translational processing. To overcome this challenge, modification of the TIMP-3 sequence to include a furin protease-cleavable pro-sequence resulted in secretion of the modified TIMP-3 protein, however, incomplete processing was observed. Based on the TIMP-3 data, the protein engineering approach was optimized and successfully applied in combination with cell engineering, the overexpression of furin, to another member of the TIMP protein family (the poorly expressed TIMP-4). Use of the described protein engineering strategy resulted in successful secretion of poorly (TIMP-4) and non-secreted (TIMP-3) targets, and presents a novel strategy to enhance the production of "difficult" recombinant targets. Biotechnol. Bioeng. 2017;114: 2348-2359. © 2017 Wiley Periodicals, Inc.

Published

2017

12. N-terminal SKIK peptide tag markedly improves expression of difficult-to-express proteins in Escherichia coli and Saccharomyces cerevisiae

Author

Hideo Nakano, Teruyo Ojima-Kato, and Satomi Nagai

Subjects

0106 biological sciences, 0301 basic medicine, Blotting, Western, Saccharomyces cerevisiae, Gene Expression, Bioengineering, Peptide, Protein tag, Biology, medicine.disease_cause, 01 natural sciences, Applied Microbiology and Biotechnology, Mice, 03 medical and health sciences, chemistry.chemical_compound, 010608 biotechnology, Escherichia coli, Protein biosynthesis, medicine, Animals, Polyacrylamide gel electrophoresis, chemistry.chemical_classification, Cell-Free System, Coomassie Brilliant Blue, Antibodies, Monoclonal, biology.organism_classification, Molecular biology, Recombinant Proteins, 030104 developmental biology, chemistry, Biochemistry, Electrophoresis, Polyacrylamide Gel, Rabbits, Oligopeptides, Biotechnology, Myc-tag

Abstract

Despite advances in microbial protein expression systems, low production of proteins remains a great concern for some genes. Here we report that the insertion of a short peptide tag, consisting of Ser-Lys-Ile-Lys (SKIK), adjacent to the start codon of genes encoding difficult-to-express proteins can increase protein expression in Escherichia coli and Saccharomyces cerevisiae. Protein expression levels of a mouse monoclonal antibody (mAb), rabbit mAbs obtained from clonal B cells, and an artificially designed peptide were significantly increased simply by the addition of the SKIK tag in E. coli systems. In particular, a ∼30-fold increase in protein production was observed for the mouse mAb, and the artificially designed peptide band became detectable in sodium dodecyl sulfate-poly acrylamide gel electrophoresis after coomassie brilliant blue staining or western blotting on adding the SKIK tag. The tag also increased the expression of tagged proteins in S. cerevisiae and an E. coli cell-free protein synthesis system. Although the mechanism of high protein expression on addition of the tag is unclear, our findings offer great benefits to biotechnology research and industry.

Published

2017

13. Metal ions-binding T4 lysozyme as an intramolecular protein purification tag compatible with X-ray crystallography

Author

Anna Dubankova, Martin Klima, Evzen Boura, Dominika Chalupska, and Adriana Baumlova

Subjects

0301 basic medicine, 030103 biophysics, Protein tag, Biology, Biochemistry, Fusion protein, 03 medical and health sciences, chemistry.chemical_compound, 030104 developmental biology, Affinity chromatography, chemistry, FLAG-tag, Protein purification, Sterol binding, Lysozyme, Molecular Biology, Myc-tag

Abstract

Phage T4 lysozyme is a well folded and highly soluble protein that is widely used as an insertion tag to improve solubility and crystallization properties of poorly behaved recombinant proteins. It has been used in the fusion protein strategy to facilitate crystallization of various proteins including multiple G protein-coupled receptors, lipid kinases, or sterol binding proteins. Here, we present a structural and biochemical characterization of its novel, metal ions-binding mutant (mbT4L). We demonstrate that mbT4L can be used as a purification tag in the immobilized-metal affinity chromatography and that, in many respects, it is superior to the conventional hexahistidine tag. In addition, structural characterization of mbT4L suggests that mbT4L can be used as a purification tag compatible with X-ray crystallography.

Published

2017

14. Production of recombinant proteins in Escherichia coli tagged with the fusion protein CusF3H+

Author

Teresa Vargas-Cortez, Xristo Zarate, Jose Ruben Morones-Ramirez, and Isaías Balderas-Rentería

Subjects

0301 basic medicine, Recombinant Fusion Proteins, Arabidopsis, Biology, Inclusion bodies, 03 medical and health sciences, Bacterial Proteins, Copper Transport Proteins, FLAG-tag, Affinity chromatography, Protein purification, Protein A/G, Basic Helix-Loop-Helix Transcription Factors, Escherichia coli, Cation Transport Proteins, 030102 biochemistry & molecular biology, Arabidopsis Proteins, Escherichia coli Proteins, Synechocystis, Fusion protein, 030104 developmental biology, Biochemistry, biology.protein, Protein G, Biotechnology, Myc-tag

Abstract

Recombinant protein expression in the bacterium Escherichia coli still is the number one choice for large-scale protein production. Nevertheless, many complications can arise using this microorganism, such as low yields, the formation of inclusion bodies, and the requirement for difficult purification steps. Most of these problems can be solved with the use of fusion proteins. Here, the use of the metal-binding protein CusF3H+ is described as a new fusion protein for recombinant protein expression and purification in E. coli. We have previously shown that CusF produces large amounts of soluble protein, with low levels of formation of inclusion bodies, and that proteins can be purified using IMAC resins charged with Cu(II) ions. CusF3H+ is an enhanced variant of CusF, formed by the addition of three histidine residues at the N-terminus. These residues then can bind Ni(II) ions allowing improved purity after affinity chromatography. Expression and purification of Green Fluorescent Protein tagged with CusF3H+ showed that the mutation did not alter the capacity of the fusion protein to increase protein expression, and purity improved considerably after affinity chromatography with immobilized nickel ions; high yields are obtained after tag-removal since CusF3H+ is a small protein of just 10 kDa. Furthermore, the results of experiments involving expression of tagged proteins having medium to large molecular weights indicate that the presence of the CusF3H+ tag improves protein solubility, as compared to a His-tag. We therefore endorse CusF3H+ as a useful alternative fusion protein/affinity tag for production of recombinant proteins in E. coli.

Published

2017

15. Proteomic analysis of contaminants in recombinant membrane hemeproteins expressed in E. coli and isolated by metal affinity chromatography

Author

M. Trawkina, Sergei A. Usanov, Ya. V. Dzichenka, G. V. Sergeev, M. A. Shapiro, Andrey Gilep, A. V. Ivanchik, A. V. Yantsevich, and T. V. Shkel

Subjects

Hemeproteins, Proteomics, Ribosomal Proteins, 0301 basic medicine, Genetic Vectors, Gene Expression, Peptide Elongation Factor Tu, medicine.disease_cause, Applied Microbiology and Biotechnology, Biochemistry, Chromatography, Affinity, Copurification, Chaperonin, 03 medical and health sciences, Affinity chromatography, FLAG-tag, Ribosomal protein, Escherichia coli, medicine, Humans, Amino Acid Sequence, Cloning, Molecular, Heat-Shock Proteins, Glutamine-Fructose-6-Phosphate Transaminase (Isomerizing), Chromatography, Flavoproteins, 030102 biochemistry & molecular biology, Chemistry, Escherichia coli Proteins, Sepharose, Peptidylprolyl Isomerase, Catalase, Recombinant Proteins, 030104 developmental biology, Proteome, Myc-tag

Abstract

Contaminating proteins have been identified by “shotgun” proteomic analysis in 14 recombinant preparations of human membrane heme- and flavoproteins expressed in Escherichia coli and purified by immobilized metal ion affinity chromatography. Immobilized metal ion affinity chromatography of ten proteins was performed on Ni2+-NTA-sepharose 6B, and the remaining four proteins were purified by ligand affinity chromatography on 2',5'-ADP-sepharose 4B. Proteomic analysis allowed to detect 50 protein impurities from E. coli. The most common contaminant was Elongation factor Tu2. It is characterized by a large dipole moment and a cluster arrangement of acidic amino acid residues that mediate the specific interaction with the sorbent. Peptidyl prolyl-cis-trans isomerase SlyD, glutamine-fructose-6-phosphate aminotransferase, and catalase HPII that contained repeating HxH, QxQ, and RxR fragments capable of specific interaction with the sorbent were identified among the protein contaminants as well. GroL/GroS chaperonins were probably copurified due to the formation of complexes with the target proteins. The Ni2+ cations leakage from the sorbent during lead to formation of free carboxyl groups that is the reason of cation exchanger properties of the sorbent. This was the putative reason for the copurification of basic proteins, such as the ribosomal proteins of E. coli and the widely occurring uncharacterized protein YqjD. The results of the analysis revealed variation in the contaminant composition related to the type of protein expressed. This is probably related to the reaction of E. coli cell proteome to the expression of a foreign protein. We concluded that the nature of the protein contaminants in a preparation of a recombinant protein purified by immobilized metal ion affinity chromatography on a certain sorbent could be predicted if information on the host cell proteome were available.

Published

2017

16. Going native: Complete removal of protein purification affinity tags by simple modification of existing tags and proteases

Author

Hui Chin Goh, Saurabh Nirantar, Farid J. Ghadessy, Radoslaw M. Sobota, and School of Biological Sciences

Subjects

0301 basic medicine, Proteases, Recombinant Fusion Proteins, medicine.medical_treatment, Native protein, Protein tag, Enforced colocalisation, Biology, Chromatography, Affinity, 03 medical and health sciences, Protein Domains, FLAG-tag, Protein purification, Escherichia coli, medicine, Affinity tags, Tandem affinity purification, Protease, 030102 biochemistry & molecular biology, 030104 developmental biology, Biochemistry, Proteolysis, Target protein, Peptide Hydrolases, Biotechnology, Myc-tag

Abstract

Protein purification typically involves expressing a recombinant gene comprising a target protein fused to a suitable affinity tag. After purification, it is often desirable to remove the affinity tag to prevent interference with downstream functions of the target protein. This is mainly accomplished by placing a protease site between the tag and the target protein. Typically, a small oligopeptide ‘stub’ C-terminal to the cleavage site remains attached to the target protein due to the requirements of sequence-specific proteases. Furthermore, steric hindrance can also limit protease efficiency. Here, we show that respectively fusing the interacting ePDZ-b/ARVCF protein-peptide pair to the target protein and a protease enables efficient processing of a minimised sequence comprising only residues N-terminal to the cleavage site. Interaction of the protein-peptide pair enforces proximity of the protease and its minimised cleavage sequence, enhancing both catalysis of a sub-optimal site and overcoming steric hindrance. This facilitates the high yield purification of fully native target proteins without recourse to specialised purification columns. NMRC (Natl Medical Research Council, S’pore) Published version

Published

2017

17. MAP Tag: A Novel Tagging System for Protein Purification and Detection

Author

Yuki Fujii, Mika K. Kaneko, and Yukinari Kato

Subjects

0301 basic medicine, Blotting, Western, Immunology, Protein domain, Antibody Affinity, Gene Expression, Antigen-Antibody Complex, Protein tag, Biology, Epitopes, Mice, 03 medical and health sciences, Protein Domains, FLAG-tag, Antibody Specificity, protein purification, Protein purification, Animals, Humans, Immunology and Allergy, Amino Acid Sequence, affinity tag, Nuclear protein, Tandem affinity purification, Membrane Glycoproteins, Staining and Labeling, Antibodies, Monoclonal, Original Articles, Molecular biology, Clone Cells, Rats, HEK293 Cells, 030104 developmental biology, Biochemistry, monoclonal antibody, COS Cells, MAP tag, Peptides, Tag system, Myc-tag

Abstract

Protein purification is an essential procedure in fields such as biochemistry, molecular biology, and biophysics. Acquiring target proteins with high quality and purity is still difficult, although several tag systems have been established for protein purification. Affinity tag systems are excellent because they possess high affinity and specificity for acquiring the target proteins. Nevertheless, further affinity tag systems are needed to compensate for several disadvantages of the presently available affinity tag systems. Herein, we developed a novel affinity tag system designated as the MAP tag system. This system is composed of a rat anti-mouse podoplanin monoclonal antibody (clone PMab-1) and MAP tag (GDGMVPPGIEDK) derived from the platelet aggregation-stimulating domain of mouse podoplanin. PMab-1 possesses high affinity and specificity for the MAP tag, and the PMab-1/MAP tag complex dissociates in the presence of the epitope peptide, indicating that the MAP tag system is suitable for protein purification. We successfully purified several proteins, including a nuclear protein, soluble proteins, and a membrane protein using the MAP tag system. The MAP tag system is very useful not only for protein purification but also in protein detection systems such as western blot and flow cytometric analyses. Taken together, these findings indicate that the MAP tag system could be a powerful tool for protein purification and detection.

Published

2016

18. Intracellular distribution of pseudorabies virus UL2 and detection of its nuclear import mechanism

Author

Meili Li, Xingmei Zou, Daixiong Chen, Jing Xiao, Weidong Gan, Yingjie Guo, Zuo Xu, Tao Peng, Yuanfang Wang, Mingsheng Cai, Xiaowen Ou, Yiwen Li, and Yangxi Deng

Subjects

0301 basic medicine, Yellow fluorescent protein, viruses, Clinical Biochemistry, Active Transport, Cell Nucleus, Pseudorabies, Importin, Biochemistry, Virus, 03 medical and health sciences, Viral Proteins, 0302 clinical medicine, Viral life cycle, Chlorocebus aethiops, Animals, Cloning, Molecular, Uracil-DNA Glycosidase, Molecular Biology, Cell Nucleus, biology, biology.organism_classification, Cell biology, 030104 developmental biology, 030220 oncology & carcinogenesis, Ran, COS Cells, biology.protein, Nuclear transport, Myc-tag

Abstract

Pseudorabies virus (PRV) UL2 (pUL2) is a multifunctional protein, which is homologous with herpes simplex virus 1 early protein UL2 (hUL2) and crucial for the viral propagation. Yet, how pUL2 executes its roles in the viral life cycle remain inadequately understood. In order to uncover its effect on the procedure of PRV infection, investigation was performed to examine the subcellular distribution of pUL2 and establish its trafficking mechanism. In the present study, enhanced yellow fluorescent protein or Myc tag fused pUL2 was transiently overexpressed in transfected cells and exhibited an absolutely nuclear accumulation without the existence of other PRV proteins. Additionally, the nuclear trafficking of pUL2 was proved to rely on Ran-, transportin-1, importin β1, importin α1, α3 and α5. Accordingly, these data will benefit the knowledge of pUL2-mediated biological effects in PRV infection cycle.

Published

2019

19. Extracellular Localisation of the C-Terminus of DDX4 Confirmed by Immunocytochemistry and Fluorescence-Activated Cell Sorting

Author

Yvonne L. Clarkson, Marie McLaughlin, Richard A. Anderson, Martin Waterfall, Evelyn E. Telfer, Emma L Weatherall, Paul A. Skehel, and Haojiang Lu

Subjects

0301 basic medicine, Cell Membrane Permeability, ovarian stem cells, Immunocytochemistry, Epitope, Article, Antibodies, DEAD-box RNA Helicases, 03 medical and health sciences, Epitopes, 0302 clinical medicine, immunocytochemistry, DDX4, Antibody Specificity, Extracellular, medicine, Humans, human, lcsh:QH301-705.5, Cell Size, 030219 obstetrics & reproductive medicine, Expression vector, Chemistry, Ovary, Reproducibility of Results, General Medicine, Cell sorting, Flow Cytometry, Embryonic stem cell, Immunohistochemistry, 3. Good health, Cell biology, Protein Transport, 030104 developmental biology, medicine.anatomical_structure, HEK293 Cells, lcsh:Biology (General), Oocytes, fluorescence-actiavted cell sorting, Female, Extracellular Space, Germ cell, fluorescence-activated cell sorting, Myc-tag

Abstract

Putative oogonial stem cells (OSCs) have been isolated by fluorescence-activated cell sorting (FACS) from adult human ovarian tissue using an antibody against DEAD-box helicase 4 (DDX4). DDX4 has been reported to be germ cell specific within the gonads and localised intracellularly. White et al. (2012) hypothesised that the C-terminus of DDX4 is localised on the surface of putative OSCs but is internalised during the process of oogenesis. This hypothesis is controversial since it is assumed that RNA helicases function intracellularly with no extracellular expression. To determine whether the C-terminus of DDX4 could be expressed on the cell surface, we generated a novel expression construct to express full-length DDX4 as a DsRed2 fusion protein with unique C- and N-terminal epitope tags. DDX4 and the C-terminal myc tag were detected at the cell surface by immunocytochemistry and FACS of non-permeabilised human embryonic kidney HEK 293T cells transfected with the DDX4 construct. DDX4 mRNA expression was detected in the DDX4-positive sorted cells by RT-PCR. This study clearly demonstrates that the C-terminus of DDX4 can be expressed on the cell surface despite its lack of a conventional membrane-targeting or secretory sequence. These results validate the use of antibody-based FACS to isolate DDX4-positive putative OSCs.

Published

2019

20. AI179 single-chain antibody recognizes the Myc tag by Western blotting

Author

Keszei, Zsofia and Picard, Didier

Subjects

biology, medicine.diagnostic_test, Myc tag, Western blot, General Medicine, Single chain, Molecular biology, law.invention, Blot, single-chain antibody, law, Recombinant DNA, biology.protein, medicine, Antibody, ddc:612, Myc-tag

Abstract

The recombinant antibody AI179 against the Myc tag detects a Myc-tagged protein exogenously expressed in human cells by Western blotting.

Published

2019

21. Multiple affinity purification of a baculovirus-derived recombinant prion protein with in vitro ability to convert to its pathogenic form

Author

Nobuko Kato, Yuichi Murayama, Morikazu Imamura, Takashi Yokoyama, Shirou Mohri, and Yoshifumi Iwamaru

Subjects

0301 basic medicine, Immunogen, animal diseases, Blotting, Western, Protein tag, Spodoptera, Biology, Biochemistry, Chromatography, Affinity, Prion Proteins, law.invention, Epitopes, Mice, 03 medical and health sciences, chemistry.chemical_compound, FLAG-tag, Affinity chromatography, law, Animals, Amino Acid Sequence, Polyhistidine-tag, Virulence, General Medicine, Molecular biology, Recombinant Proteins, nervous system diseases, 030104 developmental biology, chemistry, Recombinant DNA, Protein Misfolding Cyclic Amplification, Baculoviridae, Biotechnology, Myc-tag

Abstract

We previously showed that baculovirus-derived recombinant prion protein (Bac-PrP) can be converted to the misfolded infectious form (PrPSc) by protein misfolding cyclic amplification, an in vitro conversion technique. Bac-PrP, with post-translational modifications, would be useful for various applications such as using PrP as an immunogen for generating anti-PrP antibody, developing anti-prion drugs or diagnostic assays using in vitro conversion systems, and establishing an in vitro prion propagation model. For this purpose, highly purified Bac-PrP with in vitro conversion activity is necessary for use as a PrPC source, to minimize contamination. Furthermore, an exogenous affinity tag-free form is desirable to avoid potential steric interference by the affinity tags during the conversion process. In this study, we established purification methods for the untagged Bac-PrP under native conditions by combining exogenous double-affinity tags, namely, a polyhistidine-tag and a profinity eXact tag, with an octarepeat sequence of the N-terminal region of PrP, which has metal ion-binding affinity. The untagged Bac-PrP with near-homogeneity was obtained by three-step affinity purification, and it was shown that the final, purified Bac-PrP could convert to its pathogenic form. The presented purification procedure could be applied not only to PrP but also to other eukaryotic, recombinant proteins that require high purity and intact physiological activity.

Published

2016

22. Purification of Antibacterial CHAPK Protein Using a Self-Cleaving Fusion Tag and Its Activity Against Methicillin-Resistant Staphylococcus aureus

Author

Rezvan Moniri, Hamed Haddad Kashani, Yasaman Dasteh Goli, and Elahe Seyed Hosseini

Subjects

0301 basic medicine, 030106 microbiology, Protein tag, Biology, Microbiology, Fusion protein, Molecular biology, 03 medical and health sciences, 030104 developmental biology, Affinity chromatography, FLAG-tag, Protein splicing, Protein purification, Molecular Medicine, Intein, Molecular Biology, Myc-tag

Abstract

Therapeutic LysK-CHAP is a potent anti-staphylococcal protein that could be utilized as an antibiotic substitute. Intein-mediated protein purification is a reasonable and cost-effective method that is most recently used for recombinant therapeutic protein production. Intein (INT) is the internal parts of the protein that can be separated from the immature protein during protein splicing process. This sequence requires no specific enzyme or cofactor for separation. INT sequence and their characteristic of self-cleavage by thiol induction, temperature, and pH changes are used for protein purification. The current study presents the expression of CHAPK262 domain of LysK gene that is fused with INT/chitin-binding sequence while evaluating its purification procedure and antibacterial activity against methicillin-resistant Staphylococcus aureus (MRSA). The coding gene sequence of LysK-CHAP (CHAPK262) in pET22-b was amplified with polymerase chain reaction (PCR); the digested product was then cloned into the pTXB1 vector. Electrophoresis confirmed the cloning accuracy of the gene. The pTXB1-CHAPK262 plasmid was transformed to the Escherichia coli ER2566 (E. coli ER2566) expression strain and analyzed for expression of the recombinant protein by SDS-PAGE and Western blotting methods. Finally, CHAPK262 was purified by chitin affinity column using INT tag technology and confirmed by SDS-PAGE. Lytic activity of the purified protein was investigated by disk diffusion method. Cloning of CHAPK262 into the pTXB1 vector, which comprised INT/chitin-binding sequence, was successfully achieved. The SDS-PAGE data also revealed successful expression of the CHAPK262-INT fusion protein and Western blotting method validated the accuracy of the protein. Moreover, purification of CHAPK262 protein was induced by dithiothreitol (DTT) and confirmed by SDS-PAGE. Finally, inhibition zone in MRAS culture medium confirmed antibacterial activity of the protein. Application of intein-mediated antibacterial protein is an appropriate and streamlined method for one-step purification of CHAPK262 as a therapeutic and antibacterial protein. Self-cleaving tags like intein are cost-effective and could be used as a proper purification method for industrial purposes.

Published

2016

23. Heparin-binding peptide as a novel affinity tag for purification of recombinant proteins

Author

Jacqueline Morris, Ralph Henry, Srinivas Jayanthi, David S. McNabb, Alicia Kight, Rebekah G. Langston, Thallapuranam Krishnaswamy Suresh Kumar, and Anna E. Daily

Subjects

0301 basic medicine, Tandem affinity purification, Strep-tag, Chromatography, 030102 biochemistry & molecular biology, Arabidopsis Proteins, Heparin, Recombinant Fusion Proteins, Arabidopsis, Protein tag, Biology, Fusion protein, Chromatography, Affinity, 03 medical and health sciences, 030104 developmental biology, FLAG-tag, Affinity chromatography, Biochemistry, Protein purification, Escherichia coli, Biotechnology, Myc-tag

Abstract

Purification of recombinant proteins constitutes a significant part of the downstream processing in biopharmaceutical industries. Major costs involved in the production of bio-therapeutics mainly depend on the number of purification steps used during the downstream process. Affinity chromatography is a widely used method for the purification of recombinant proteins expressed in different expression host platforms. Recombinant protein purification is achieved by fusing appropriate affinity tags to either N- or C- terminus of the target recombinant proteins. Currently available protein/peptide affinity tags have proved quite useful in the purification of recombinant proteins. However, these affinity tags suffer from specific limitations in their use under different conditions of purification. In this study, we have designed a novel 34-amino acid heparin-binding affinity tag (HB-tag) for the purification of recombinant proteins expressed in Escherichia coli (E. coli) cells. HB-tag fused recombinant proteins were overexpressed in E. coli in high yields. A one-step heparin-Sepharose-based affinity chromatography protocol was developed to purify HB-fused recombinant proteins to homogeneity using a simple sodium chloride step gradient elution. The HB-tag has also been shown to facilitate the purification of target recombinant proteins from their 8 M urea denatured state(s). The HB-tag has been demonstrated to be successfully released from the fusion protein by an appropriate protease treatment to obtain the recombinant target protein(s) in high yields. Results of the two-dimensional NMR spectroscopy experiments indicate that the purified recombinant target protein(s) exist in the native conformation. Polyclonal antibodies raised against the HB-peptide sequence, exhibited high binding specificity and sensitivity to the HB-fused recombinant proteins (∼10 ng) in different crude cell extracts obtained from diverse expression hosts. In our opinion, the HB-tag provides a cost-effective, rapid, and reliable avenue for the purification of recombinant proteins in heterologous hosts.

Published

2016

24. A novel self-cleavable tag Zbasic–∆I-CM and its application in the soluble expression of recombinant human interleukin-15 in Escherichia coli

Author

Huanhuan Chen, Zhang Lei, Jiaxian Wang, Hua Jiang, Yueqing Xie, Junsheng Chen, Lei Feng, Han Luo, Ninghuan Li, Huili Lu, Jianwei Zhu, Chencen Zhu, and Shi Siwei

Subjects

0106 biological sciences, 0301 basic medicine, Recombinant Fusion Proteins, Protein tag, Biology, medicine.disease_cause, 01 natural sciences, Applied Microbiology and Biotechnology, Mass Spectrometry, Biopharmaceutics, Inteins, law.invention, Recombinant Human Interleukin-15, 03 medical and health sciences, law, 010608 biotechnology, Escherichia coli, medicine, Humans, Interleukin-15, Chromatography, Mycobacterium tuberculosis, General Medicine, Hydrogen-Ion Concentration, Fusion protein, 030104 developmental biology, Biopharmaceutical, Solubility, Biochemistry, Recombinant DNA, Intein, Chromatography, Liquid, Biotechnology, Myc-tag

Abstract

Soluble expression of recombinant therapeutic proteins in Escherichia coli (E. coli) has been a challenging task in biopharmaceutical development. In this study, a novel self-cleavable tag Zbasic–intein has been constructed for the soluble expression and purification of a recombinant cytokine, human interleukin-15 (IL-15). We screened several solubilizing tags fused with the self-cleavable Mycobacterium tuberculosis recA mini-intein ∆I-CM and demonstrated that Zbasic tag can significantly improve the solubility of the product with correspondent to the intein activity. The fusion protein “Zbasic–∆I-CM–IL-15” was expressed with high solubility and easily enriched by the cost-effective cation-exchange chromatography. The self-cleavage of the fusion tag Zbasic–∆I-CM was then induced by a pH shift, with an activation energy of 7.48 kcal/mol. The mature IL-15 with natural N-terminus was released and further purified by hydrophobic interaction and anion-exchange chromatography. High-resolution reverse-phase high-performance liquid chromatography and mass spectrometry analysis confirmed that the product was of high purity and correct mass. With a CTLL-2 cell proliferation-based assay, the EC50 was evaluated to be of about 0.126 ng/mL, similar to the product in clinical trials. By avoiding the time-consuming denaturing-refolding steps in previously reported processes, the current method is efficient and cost-effective. The novel tag Zbasic–∆I-CM can be potentially applied to large-scale manufacturing of recombinant human cytokines as well as other mammalian-sourced proteins in E. coli.

Published

2016

25. Evaluation of employing poly-lysine tags versus poly-histidine tags for purification and characterization of recombinant copper-binding proteins

Author

Zhiguang Xiao, Ashwinie A. Ukuwela, Chathuri J. K. Wijekoon, and Anthony G. Wedd

Subjects

0106 biological sciences, 0301 basic medicine, Cations, Divalent, Recombinant Fusion Proteins, Gene Expression, Protein tag, Pseudomonas fluorescens, 01 natural sciences, Biochemistry, Chromatography, Affinity, Inorganic Chemistry, 03 medical and health sciences, FLAG-tag, 010608 biotechnology, Protein purification, Escherichia coli, Metalloprotein, Histidine, Polylysine, Cloning, Molecular, Tandem affinity purification, chemistry.chemical_classification, Staining and Labeling, Chemistry, Cations, Monovalent, Chromatography, Ion Exchange, Isotope-coded affinity tag, Carboxypeptidase B, 030104 developmental biology, Carrier Proteins, Copper, Myc-tag

Abstract

Quantitative characterization of metalloproteins at molecular and atomic levels generally requires tens of milligrams of highly purified samples, a situation frequently challenged by problems in generating unmodified native forms. A variety of affinity tags, such as the popular poly-histidine tag, have been developed to facilitate purification but they generally rely on expensive affinity resins and their presence may interfere with protein characterization. This paper documents that addition of a poly-lysine tag to the C-terminus enables, for the copper-binding proteins examined, ready purification in large scale via cost-effective cation-exchange chromatography. The tag may be removed readily by the enzyme carboxypeptidase B to generate the native protein with no extra residues. However, this cleavage step is normally not necessary since the poly-lysine tag is shown to have no detectable affinity for either Cu(I) or Cu(II) and imposes no interference to the copper binding properties of the target proteins. In contrast, the poly-histidine tag possesses a sub-picomolar affinity for Cu(I) and -nanomolar affinity for Cu(II) and may need to be removed for reliable characterization of the target proteins. These conclusions may be extended to the study of other metallo-proteins and metallo-enzymes.

Published

2016

26. A dual protease approach for expression and affinity purification of recombinant proteins

Author

David S. Waugh and Sreejith Raran-Kurussi

Subjects

0301 basic medicine, Rhinovirus, Recombinant Fusion Proteins, medicine.medical_treatment, Biophysics, Biochemistry, Article, Maltose-Binding Proteins, law.invention, Viral Proteins, 03 medical and health sciences, Maltose-binding protein, Affinity chromatography, FLAG-tag, law, Endopeptidases, Tobacco, Escherichia coli, medicine, Molecular Biology, Tandem affinity purification, Chromatography, Protease, biology, Tobacco etch virus, 3C Viral Proteases, Cell Biology, biology.organism_classification, Cysteine Endopeptidases, 030104 developmental biology, biology.protein, Recombinant DNA, Myc-tag

Abstract

We describe a new method for affinity purification of recombinant proteins using a dual protease protocol. Escherichia coli maltose binding protein (MBP) is employed as an N-terminal tag to increase the yield and solubility of its fusion partners. The MBP moiety is then removed by rhinovirus 3C protease, prior to purification, to yield an N-terminally His6-tagged protein. Proteins that are only temporarily rendered soluble by fusing them to MBP are readily identified at this stage because they will precipitate after the MBP tag is removed by 3C protease. The remaining soluble His6-tagged protein, if any, is subsequently purified by immobilized metal affinity chromatography (IMAC). Finally, the N-terminal His6 tag is removed by His6-tagged tobacco etch virus (TEV) protease to yield the native recombinant protein, and the His6-tagged contaminants are removed by adsorption during a second round of IMAC, leaving only the untagged recombinant protein in the column effluent. The generic strategy described here saves time and effort by removing insoluble aggregates at an early stage in the process while also reducing the tendency of MBP to "stick" to its fusion partners during affinity purification.

Published

2016

27. Heterologous expression of Hordeum vulgare protein Z4 in Pichia pastoris shows increased structural stability

Author

Qi Li, Xueliang Wang, Yupeng Han, Yongxian Li, and Jinjing Wang

Subjects

0106 biological sciences, 0301 basic medicine, biology, Chemistry, Bioengineering, biology.organism_classification, 01 natural sciences, Applied Microbiology and Biotechnology, Biochemistry, Pichia pastoris, 03 medical and health sciences, 030104 developmental biology, FLAG-tag, Affinity chromatography, Chemical engineering, 010608 biotechnology, Protein A/G, biology.protein, Hordeum vulgare, Protein G, Heterologous expression, Myc-tag

Abstract

Protein Z4, an abundant of serpin storage proteins of Hordeum vulgare , is one major factor that benefits the stability of beer foam. In this study, protein Z4 from Canadian malt Metcalfe was cloned and expressed in Pichia pastoris . The glycosylated 45 kDa of recombinant protein Z4 was purified by Ni-NTA affinity column. The secondary structure of recombinant protein Z4 was detected via Circular Dichroism (CD) and Fourier Transform Infrared Spectroscopy (FTIR), and β-sheets and β-turns were the main structure of recombinant protein Z4. A few structural differences between recombinant protein Z4 and protein Z4 from malt were also analyzed, that more obvious α-helical structure and more S-H contents were detected in recombinant protein Z4. Meanwhile, higher structural stability of recombinant protein Z4 was also observed after incubating the samples in a wide range of temperature, pH and ethanol. These results confirmed the positive relationship between modifications by saccharides and high structural stability of recombinant protein Z4.

Published

2016

28. Production of recombinant human interleukin-38 and its inhibitory effect on the expression of proinflammatory cytokines in THP-1 cells

Author

Mingcai Li, Yan Li, Mi Zhou, Qiaoyan Gao, Xiuhe Pan, and Xianli Yuan

Subjects

0301 basic medicine, medicine.medical_treatment, Monocyte, Biophysics, Interleukin, Biology, Fusion protein, Molecular biology, law.invention, Proinflammatory cytokine, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, Cytokine, medicine.anatomical_structure, Affinity chromatography, Biochemistry, Structural Biology, law, 030220 oncology & carcinogenesis, medicine, Recombinant DNA, Myc-tag

Abstract

Interleukin (IL)-38 is the latest member of the IL-1 cytokine family. However, as a result of lacking efficient method to generate relatively large quantity of IL-38, its precise functions are poorly understood. In the present study, the cloning, expression, purification, and activity analysis of recombinant human IL-38 was described. Human IL-38 cDNA was cloned into the prokaryotic expression vector pET-44. The recombinant IL-38 containing a C-hexahistidine tag was expressed in Escherichia coli BL21 (DE3) which induced by isopropyl-β-D-thiogalactoside. The expressed fusion protein was purified by Ni-NTA affinity chromatography. IL-38 protein was largely found in the soluble fraction. The purified IL-38 appeared a single band on SDS-PAGE, the yield of IL-38 was 4 mg from 1 L of bacterial culture, and the purity was more than 98% with low endotoxin level (

Published

2016

29. A Novel Recombinant DNA System for High Efficiency Affinity Purification of Proteins in Saccharomyces cerevisiae

Author

Philip J. Smaldino, Brian H Carrick, Linxuan Hao, and David R. Engelke

Subjects

0301 basic medicine, Recombinant Fusion Proteins, 030303 biophysics, Saccharomyces cerevisiae, DNA, Recombinant, QH426-470, Biology, Investigations, Chromatography, Affinity, law.invention, chemistry.chemical_compound, 03 medical and health sciences, FLAG-tag, Affinity chromatography, law, Protein purification, Endopeptidases, Genetics, TEV protease, Cellulose, Molecular Biology, Genetics (clinical), 030304 developmental biology, CBM3, 0303 health sciences, 030102 biochemistry & molecular biology, Chemistry, myc epitope, affinity purification, biology.organism_classification, Cellulose binding, Molecular biology, Phosphoglycerate Kinase, 030104 developmental biology, Biochemistry, CelTag, Saccharomyces cerevisiae protein purification, Recombinant DNA, DNA construct, DNA, Myc-tag

Abstract

Isolation of endogenous proteins from Saccharomyces cerevisiae has been facilitated by inserting encoding polypeptide affinity tags at the C-termini of chromosomal open reading frames (ORFs) using homologous recombination of DNA fragments. Tagged protein isolation is limited by a number of factors, including high cost of affinity resins for bulk isolation and low concentration of ligands on the resin surface, leading to low isolation efficiencies and trapping of contaminants. To address this, we have created a recombinant “CelTag” DNA construct from which PCR fragments can be created to easily tag C-termini of S. cerevisiae ORFs using selection for a nat1 marker. The tag has a C-terminal cellulose binding module to be used in the first affinity step. Microgranular cellulose is very inexpensive and has an effectively continuous ligand on its surface, allowing rapid, highly efficient purification with minimal background. Cellulose-bound proteins are released by specific cleavage of an included site for TEV protease, giving nearly pure product. The tag can be lifted from the recombinant DNA construct either with or without a 13x myc epitope tag between the target ORF and the TEV protease site. Binding of CelTag protein fusions to cellulose is stable to high salt, nonionic detergents, and 1 M urea, allowing stringent washing conditions to remove loosely associated components, as needed, before specific elution. It is anticipated that this reagent could allow isolation of protein complexes from large quantities of yeast extract, including soluble, membrane-bound, or nucleic acid-associated assemblies.

Published

2015

30. Anti-c-Myc Tag (9E10) Affinity Gel Protocol v1

Author

Kelsey Knight

Subjects

Chemistry, Molecular biology, Myc-tag

Abstract

Catalog Number:658502Storage Temperature:2°C-8°CProduct DescriptionAnti-c-Myc Tag (9E10) Affinity Gel consists of anti-c-myc monoclonal antibody (clone 9E10), covalently immobilized onto 6% high density glyoxal agarose beads. The affinity resin can be used in affinity purifying and immunoprecipitation of c-Myc-tagged fusion protein.Binding SpecificityMouse monoclonal antibody 9E10 recognizes the c-myc epitope N-EQKLSEEDL-C and is purified through Protein G chromatography. The antibody conjugated affinity resin can bind to epitope at N-terminal, C-terminal, and internal locations of a fusion protein. The binding capacity is greater than 0.5mg per ml of c-myc agarose resin.ReagentAnti-c-Myc Agarose Affinity Gel is supplied as a 50% suspension in phosphate-buffered saline, pH 7.2, containing 0.09% sodium azide.Precautions and DisclaimerThis product is for research use only. Please consult the Material Safety Data Sheet for information regarding hazards and safe handling practices.Storage/StabilityAnti-c-Myc Agarose Affinity Gel should be stored between 2°C and 8°C for maximum stability. The unopened product is stable for one year when stored as indicated. After use, the resin should be regenerated and stored in TBS or PBS buffer (pH 7.2) containing 0.09% sodium azide.

Published

2018

31. Membrane-bound and soluble forms of an NMDA receptor extracellular domain retain epitopes targeted in auto-immune encephalitis

Author

Scott K. Dessain, Rashmi Sharma, Amy Rattelle, David A. Lynch, Rama Devudu Puligedda, and Fetweh H. Al-Saleem

Subjects

Monoclonal antibody, 0301 basic medicine, medicine.drug_class, lcsh:Biotechnology, Autoimmunity, Recombinant protein expression, Immunofluorescence, Receptors, N-Methyl-D-Aspartate, Epitope, Cell Line, Epitopes, 03 medical and health sciences, 0302 clinical medicine, Antigen, lcsh:TP248.13-248.65, Endopeptidases, medicine, Humans, TEV protease, ANRE, Autoimmune encephalitis, biology, medicine.diagnostic_test, Methodology Article, Antibodies, Monoclonal, Membrane Proteins, NMDA receptor, Fusion protein, Molecular biology, Recombinant Proteins, 3. Good health, HEK293 Cells, 030104 developmental biology, Anti-N-methyl-D-aspartate receptor encephalitis, biology.protein, Antibody, Conformational epitope, 030217 neurology & neurosurgery, Biotechnology, Myc-tag

Abstract

Background Anti-NMDA receptor encephalitis (ANRE) is a potentially lethal disease attributed to auto-antibodies against the N-methyl-D-aspartate receptor (NMDAR). Full recovery is possible if therapy is initiated early in the disease course. Detection of ANRE antibodies in the cerebrospinal fluid (CSF) is essential for diagnosis. The assays for ANRE-associated IgGs often rely on cells transiently transfected with NMDAR genes. A cell line that stably expresses pathogenic NMDAR epitopes could improve standardization of the assays and provide antigen that could be used in commercial solid state assay systems. Results We expressed the amino terminal domain (ATD) of the GluN1 NMDAR subunit (NR1) as a fusion protein on the outer plasma membrane of 293T cells, creating a stable cell population (293T-ATD) that is recognized by ANRE patient monoclonal antibodies in flow cytometry and immunofluorescence assays. The ATD fusion protein also contains a Myc tag and a 6XHIS tag, which provide functionality for immunoassays and antigen purification, and a TEV protease site, which allows the ATD domain to be specifically released from the cells in essentially pure form. ATD mobilized from the 293T ATD cell line maintained the pathogenic ANRE epitopes in ELISA binding assays. CSF (3/4) and sera (4/4) from ANRE patients also bound the 293T-ATD cell line, whereas normal CSF and sera did not. Conclusions The 293T-ATD cell line is potentially adaptable to a variety of formats to identify antibodies associated with ANRE, including cell-based and soluble antigen formats, and demonstrates a useful method to produce complex proteins for research, drug discovery, and clinical diagnosis. Electronic supplementary material The online version of this article (10.1186/s12896-018-0450-1) contains supplementary material, which is available to authorized users.

Published

2018

32. Purification of recombinant proteins by chemical removal of the affinity tag

Author

Carole Rais-Beghdadi, Nicolas Fasel, Mario Roggero, and Christophe Reymond

Subjects

medicine.medical_treatment, Molecular Sequence Data, Plasmodium falciparum, Protozoan Proteins, Bioengineering, Biology, Applied Microbiology and Biotechnology, Biochemistry, Chromatography, Affinity, Mass Spectrometry, chemistry.chemical_compound, FLAG-tag, Affinity chromatography, Escherichia coli, medicine, Animals, Histidine, Amino Acid Sequence, Cyanogen Bromide, Molecular Biology, Tandem affinity purification, Chromatography, Protease, General Medicine, Fusion protein, Isotope-coded affinity tag, Cyanogen Bromide/chemistry, Histidine/chemistry, Protozoan Proteins/biosynthesis, Protozoan Proteins/chemistry, Recombinant Proteins/biosynthesis, Recombinant Proteins/isolation & purification, Recombinant Proteins, chemistry, Cyanogen bromide, Biotechnology, Myc-tag

Abstract

The efficient removal of a N- or C-terminal purification tag from a fusion protein is necessary to obtain a protein in a pure and active form, ready for use in human or animal medicine. Current techniques based on enzymatic cleavage are expensive and result in the presence of additional amino acids at either end of the proteins, as well as contaminating proteases in the preparation. Here we evaluate an alternative method to the one-step affinity/protease purification process for large-scale purification. It is based upon the cyanogen bromide (CNBr) cleavage at a single methionine placed in between a histidine tag and a Plasmodium falciparum antigen. The C-terminal segment of the circumsporozoite polypeptide was expressed as a fusion protein with a histidine tag in Escherichia coli purified by Ni-NAT agarose column chromatography and subsequently cleaved by CNBr to obtain a polypeptide without any extraneous amino acids derived from the cleavage site or from the affinity purification tag. Thus, a recombinant protein is produced without the need for further purification, demonstrating that CNBr cleavage is a precise, efficient, and low-cost alternative to enzymatic digestion, and can be applied to large-scale preparations of recombinant proteins.

Published

2018

33. Identification of Proteolytic Cleavage Sites of EphA2 by Membrane Type 1 Matrix Metalloproteinase on the Surface of Cancer Cells

Author

Masaaki Oyama, Hiroko Kozuka-Hata, Motoharu Seiki, Keiji Kikuchi, and Naohiko Koshikawa

Subjects

0301 basic medicine, chemistry.chemical_classification, Chemistry, Cell, Matrix metalloproteinase, Cleavage (embryo), Trypsin, Amino acid, 03 medical and health sciences, 030104 developmental biology, medicine.anatomical_structure, Affinity chromatography, Biochemistry, Membrane protein, medicine, Myc-tag, medicine.drug

Abstract

Proteolytic cleavage of membrane proteins can alter their functions depending on the cleavage sites. We recently demonstrated that membrane type 1 matrix metalloproteinase (MT1-MMP ) converts the tumor suppressor EphA2 into an oncogenic signal transducer through EphA2 cleavage. The cleaved EphA2 fragment that remains at the cell surface may be a better target for cancer therapy than intact EphA2. To analyze the cleavage site(s) of EphA2, we purified the fragments from tumor cells expressing MT1-MMP and Myc- and 6× His-tagged EphA2 by two-step affinity purification . The purified fragment was digested with trypsin to generate proteolytic peptides , and the amino acid sequences of these peptides were determined by nano-LC-mass spectrometry to identify the MT1-MMP-mediated cleavage site(s) of EphA2.

Published

2018

34. Purification of a recombinant glutathione transferase from the causative agent of hydatidosis,Echinococcus granulosus

Author

Andrea L. Fleitas, Matías N. Möller, Ana Denicola, and Lía M. Randall

Subjects

0301 basic medicine, Chromatography, Protease, biology, medicine.medical_treatment, 05 social sciences, Quantitative proteomics, 050301 education, biology.organism_classification, Biochemistry, Enzyme assay, law.invention, 03 medical and health sciences, 030104 developmental biology, FLAG-tag, law, Protein purification, medicine, Recombinant DNA, biology.protein, Echinococcus granulosus, 0503 education, Molecular Biology, Myc-tag

Abstract

This practical class activity was designed to introduce students to recombinant protein expression and purification. The principal goal is to shed light on basic aspects concerning recombinant protein production, in particular protein expression, chromatography methods for protein purification, and enzyme activity as a tool to evaluate purity and conformation of the recombinant product. Herein, we describe the purification of a glutathione transferase from the human parasite Echinococcus granulosus (EgGST1), the causative agent of hydatidosis. EgGST1 is expressed fused to a histidine tag and is purified by immobilized metal affinity chromatography. Protein quantification based on direct (UV absorbance) and indirect (colorimetric) methods are used and discussed. A simple colorimetric assay is used to measure GST activity and special emphasis is put on how to use these measurements to follow protein purification yields, its enrichment and its correct folding along the purification process. EgGST1 is easily expressed with high yields, purified in absence of protease inhibitors and proved to be robust concerning enzyme activity and protein integrity on a 1 week practical activity.

Published

2015

35. Improving recombinant protein production in the Chlamydomonas reinhardtii chloroplast using vivid Verde Fluorescent Protein as a reporter

Author

Saul Purton, Frank Baganz, and Stephanie Braun-Galleani

Subjects

Chloroplasts, Chlamydomonas reinhardtii, medicine.disease_cause, Protein Engineering, Applied Microbiology and Biotechnology, Chloroplast, Fluorescence, law.invention, Reporter protein, law, Genes, Reporter, medicine, Promoter Regions, Genetic, Escherichia coli, Gene, Research Articles, biology, General Medicine, Protein engineering, biology.organism_classification, Molecular biology, Recombinant Proteins, Luminescent Proteins, Biochemistry, Chaperone (protein), biology.protein, Recombinant DNA, Molecular Medicine, Protein expression, Myc-tag, Research Article, Biotechnology

Abstract

Microalgae have potential as platforms for the synthesis of high‐value recombinant proteins due to their many beneficial attributes including ease of cultivation, lack of pathogenic agents, and low‐cost downstream processing. However, current recombinant protein levels are low compared to other microbial platforms and stable insertion of transgenes is available in only a few microalgal species. We have explored different strategies aimed at increasing growth rate and recombinant protein production in the Chlamydomonas reinhardtii chloroplast. A novel fluorescent protein (vivid Verde Fluorescent Protein, VFP) was expressed under the control of the native atpA promoter/5'UTR element. VFP levels were detected by western blotting, with increased protein levels observed when co‐expressed with a gene encoding the Escherichia coli Spy chaperone. We used these transformant lines to study the effect of temperature, light and media on recombinant protein production and cell growth. VFP levels and fluorescence, assessed by flow cytometry, allowed a determination of improved cultivation conditions as 30°C under mixotrophic mode. These conditions were tested for the accumulation of an antimicrobial endolysin (Cpl‐1) of potential commercial interest, observing that the outcome obtained for VFP could not be easily replicated for Cpl‐1. This study suggests that recombinant protein expression is product‐specific and needs to be optimized individually.

Published

2015

36. Recombinant expression and purification of a MAP30-cell penetrating peptide fusion protein with higher anti-tumor bioactivity

Author

Jian Zhao, Qiang Lv, Yv-Ting Lu, Xu-Zhong Yang, Yan-Hua Lu, Fu-Jun Wang, and Fu Longyun

Subjects

biology, Recombinant Fusion Proteins, Ribosome-inactivating protein, Antineoplastic Agents, Cell-Penetrating Peptides, Fusion protein, Molecular biology, law.invention, Ribosome Inactivating Proteins, Type 2, FLAG-tag, Biochemistry, Affinity chromatography, law, Neoplasms, Protein A/G, biology.protein, Recombinant DNA, Humans, Protein G, HeLa Cells, Biotechnology, Myc-tag

Abstract

MAP30 (Momordica Antiviral Protein 30 Kd), a single-stranded type-I ribosome inactivating protein, possesses versatile biological activities including anti-tumor abilities. However, the low efficiency penetrating into tumor cells hampers the tumoricidal effect of MAP30. This paper describes MAP30 fused with a human-derived cell penetrating peptide HBD which overcome the low uptake efficiency by tumor cells and exhibits higher anti-tumor bioactivity. MAP30 gene was cloned from the genomic DNA of Momordica charantia and the recombinant plasmid pET28b-MAP30-HBD was established and transferred into Escherichia coli BL21 (DE3). The recombinant MAP30-HBD protein (rMAP30-HBD) was expressed in a soluble form after being induced by 0.5mM IPTG for 14h at 15°C. The recombinant protein was purified to greater than 95% purity with Ni-NTA affinity chromatography. The rMAP30-HBD protein not only has topological inactivation and protein translation inhibition activity but also showed significant improvements in cytotoxic activity compared to that of the rMAP30 protein without HBD in the tested tumor cell lines, and induced higher apoptosis rates in HeLa cells analyzed by Annexin V-FITC with FACS. This paper demonstrated a new method for improving MAP30 protein anti-tumor activity and might have potential applications in cancer therapy area.

Published

2015

37. Pharmacological profile of a bifunctional ligand of the formyl peptide receptor1 fused to the myc epitope

Author

Xavier Charest-Morin, François Marceau, Caroline Roy, and Maria J.G. Fernandes

Subjects

Neutrophils, medicine.drug_class, Recombinant Fusion Proteins, media_common.quotation_subject, Immunology, Peptide, Ligands, Monoclonal antibody, Epitope, Cell Line, Proto-Oncogene Proteins c-myc, Epitopes, medicine, Humans, Immunology and Allergy, Myeloid Cells, Internalization, media_common, Pharmacology, chemistry.chemical_classification, biology, Antibodies, Monoclonal, Cell Differentiation, Stereoisomerism, Receptor-mediated endocytosis, Ligand (biochemistry), Receptors, Formyl Peptide, Molecular biology, Endocytosis, N-Formylmethionine Leucyl-Phenylalanine, chemistry, biology.protein, Antibody, Protein Binding, Myc-tag

Abstract

In human peripheral blood neutrophils or in myeloid PLB-985 cells differentiated towards a neutrophil-like phenotype, the peptide N-formyl-L-norleucyl-L-leucyl-L-phenylalanyl-L-norleucyl-L-tyrosyl-L-leucyl-fluorescein isothiocyanate (f-Nle-Leu-Phe-Nle-Tyr-Lys-FITC) binds to and activates formyl peptide receptor1 (FPR1) and is submitted to receptor-mediated endocytosis (microscopy, cytofluorometry). This peptide may be considered a C-terminally extended version of f-Met-Leu-Phe which carries a fluorescent cargo into cells. By analogy to other peptide hormones for which we have evaluated epitope-tagged agonists as carriers of antibody cargoes, we have designed and evaluated f-Nle-Leu-Phe-Nle-Tyr-Lys-myc, C-terminally extended with the 10-residue myc tag. This peptide is as potent as f-Met-Leu-Phe to compete for f-Nle-Leu-Phe-Nle-Tyr-Lys-FITC uptake by PLB-985 cells, but did not mediate (10-1000nM) the internalization of the fluorescent anti-myc monoclonal antibody 4A6 added to the extracellular fluid at ~7nM (microscopy). The nonfluorescent version of the antibody (28nM) acts as a pre-receptor antagonist of f-Nle-Leu-Phe-Nle-Tyr-Lys-myc, but not of f-Met-Leu-Phe (superoxide release assay in differentiated PLB-985 cells). A further prolonged analog, f-Nle-Leu-Phe-Nle-Tyr-Lys-(Asn-Gly)5-myc, designed to decrease the possible steric hindrance between FPR1 and the bound anti-myc antibody, has little affinity for the receptor, precluding a direct assessment of this issue. Thus, the relatively low-affinity anti-myc antibody used at a high concentration functionally behaves as a selective pre-receptor antagonist of the agonist f-Nle-Leu-Phe-Nle-Tyr-Lys-myc.

Published

2015

38. Microbial Transglutaminase and c-myc-Tag: A Strong Couple for the Functionalization of Antibody-Like Protein Scaffolds from Discovery Platforms

Author

Patrick Dennler, Eliane Fischer, Laura K. Bailey, Roger Schibli, and Philipp R. Spycher

Subjects

Immunoconjugates, Mice, SCID, 01 natural sciences, Biochemistry, Antibodies, Cell Line, Proto-Oncogene Proteins c-myc, Mice, 03 medical and health sciences, Fluorescence microscope, Animals, Humans, Amino Acid Sequence, Molecular Biology, Peptide sequence, Fluorescent Dyes, 030304 developmental biology, chemistry.chemical_classification, Mice, Inbred ICR, 0303 health sciences, Isopeptide bond, Transglutaminases, Bioconjugation, 010405 organic chemistry, Chemistry, Organic Chemistry, Neoplasms, Experimental, Cell sorting, Recombinant Proteins, 0104 chemical sciences, Molecular Probes, Molecular Medicine, Surface modification, Female, Myc-tag, Conjugate

Abstract

Antibody-like proteins selected from discovery platforms are preferentially functionalized by site-specific modification as this approach preserves the binding abilities and allows a side-by-side comparison of multiple conjugates. Here we present an enzymatic bioconjugation platform that targets the c-myc-tag peptide sequence (EQKLISEEDL) as a handle for the site-specific modification of antibody-like proteins. Microbial transglutaminase (MTGase) was exploited to form a stable isopeptide bond between the glutamine on the c-myc-tag and various primary-amine-functionalized substrates. We attached eight different functionalities to a c-myc-tagged antibody fragment and used these bioconjugates for downstream applications such as protein multimerization, immobilization on surfaces, fluorescence microscopy, fluorescence-activated cell sorting, and in vivo nuclear imaging. The results demonstrate the versatility of our conjugation strategy for transforming a c-myc-tagged protein into any desired probe.

Published

2015

39. Simple and Efficient Purification of Recombinant Proteins Using the Heparin‐Binding Affinity Tag

Author

Srinivas Jayanthi, Ravi Kumar Gundampati, and Thallapuranam Krishnaswamy Suresh Kumar

Subjects

0301 basic medicine, Recombinant Fusion Proteins, Genetic Vectors, Gene Expression, Protein tag, Sodium Chloride, Biochemistry, Article, Chromatography, Affinity, law.invention, 03 medical and health sciences, Affinity chromatography, FLAG-tag, Structural Biology, law, Escherichia coli, Amino Acid Sequence, Cloning, Molecular, Tandem affinity purification, Chromatography, 030102 biochemistry & molecular biology, Chemistry, Sepharose, Blood Proteins, Chromatography, Agarose, Fusion protein, Isotope-coded affinity tag, 030104 developmental biology, Recombinant DNA, Carrier Proteins, Antimicrobial Cationic Peptides, Myc-tag

Abstract

Heparin, a member of the glycosaminoglycan family, is known to interact with more than 400 different types of proteins. For the past few decades, significant progress has been made to understand the molecular details involved in heparin-protein interactions. Based on the structural knowledge available from the FGF1-heparin interaction studies, we have designed a novel heparin-binding peptide (HBP) affinity tag that can be used for the simple, efficient, and cost-effective purification of recombinant proteins of interest. Purification of recombinant proteins using the HBP tag can be achieved using a simple sodium chloride gradient. In addition, owing to the high density of positive charges on the HBP tag, recombinant target proteins are preferably expressed in their soluble forms. Further, the purification of HBP-fused proteins/peptides can also be achieved in the presence of chemical denaturants like urea. Additionally, polyclonal antibodies raised against the affinity tag can be used to detect HBP-fused target proteins with high sensitivity. Given these properties, we believe that the HBP tag will be enthusiastically used by researchers for the purification of recombinant proteins.

Published

2017

40. Recombinant human interleukin-12 is the second example of a C-mannosylated protein

Author

Daniel Hess, Jan Hofsteenge, Marie-Agnès Doucey, and Marcel J. J. Blommers

Subjects

Glycosylation, Magnetic Resonance Spectroscopy, RNase P, Peptide, CHO Cells, In Vitro Techniques, Biochemistry, Mannosyltransferases, law.invention, Substrate Specificity, FLAG-tag, law, Cricetinae, Animals, Humans, Amino Acid Sequence, chemistry.chemical_classification, B-Lymphocytes, Chemistry, Tryptophan, Interleukin-12, Peptide Fragments, Recombinant Proteins, carbohydrates (lipids), Mannosylation, Interleukin 12, Recombinant DNA, Mannose, Myc-tag

Abstract

The beta-chain of human interleukin 12 (IL-12) contains at position 319-322, the sequence Trp-x-x-Trp. In human RNase 2 this is the recognition motif for a new, recently discovered posttranslational modification, i.e., the C-glycosidic attachment of a mannosyl residue to the side chain of tryptophan. Analysis of C-terminal peptides of recombinant IL-12 (rHuIL-12) by mass spectrometry and NMR spectroscopy revealed that Trp-319beta is (partially) C-mannosylated. This finding was extended by in vitro mannosylation experiments, using a synthetic peptide derived from the same region of the protein as an acceptor. Furthermore, human B-lymphoblastoid cells, which secrete IL-12, were found to contain an enzyme that carries out the C-mannosylation reaction. This shows that nonrecombinant IL-12 is potentially C-mannosylated as well. This is only the second report on a C-mannosylated protein. However, the occurrence of the C-mannosyltransferase activity in a variety of cells and tissues, and the presence of the recognition motif in many proteins indicate that more C-mannosylated proteins may be found.

Published

2017

41. High-level expression of soluble recombinant proteins in Escherichia coli using an HE-maltotriose-binding protein fusion tag

Author

Jiang Wang, Bei-Bei Chu, Ying-Qian Han, Guo-Yu Yang, Yujie Guo, Guo Wanying, and Bing-Qian Su

Subjects

0301 basic medicine, Recombinant Fusion Proteins, Gene Expression, Protein tag, medicine.disease_cause, Chromatography, Affinity, Maltose-Binding Proteins, 03 medical and health sciences, FLAG-tag, Endopeptidases, medicine, Escherichia coli, Histidine, Cloning, Molecular, Tandem affinity purification, biology, Tobacco etch virus, Protein Stability, Binding protein, fungi, biology.organism_classification, Fusion protein, Molecular biology, Pyrococcus furiosus, 030104 developmental biology, Biochemistry, Solubility, Oligopeptides, Trisaccharides, Biotechnology, Myc-tag, Plasmids, Protein Binding

Abstract

Recombinant proteins are commonly expressed in prokaryotic expression systems for large-scale production. The use of genetically engineered affinity and solubility enhancing fusion proteins has increased greatly in recent years, and there now exists a considerable repertoire of these that can be used to enhance the expression, stability, solubility, folding, and purification of their fusion partner. Here, a modified histidine tag (HE) used as an affinity tag was employed together with a truncated maltotriose-binding protein (MBP; consisting of residues 59–433) from Pyrococcus furiosus as a solubility enhancing tag accompanying a tobacco etch virus protease-recognition site for protein expression and purification in Escherichia coli . Various proteins tagged at the N-terminus with HE-MBP(Pyr) were expressed in E. coli BL21(DE3) cells to determine expression and solubility relative to those tagged with His6-MBP or His6-MBP(Pyr). Furthermore, four HE-MBP(Pyr)-fused proteins were purified by immobilized metal affinity chromatography to assess the affinity of HE with immobilized Ni 2+ . Our results showed that HE-MBP(Pyr) represents an attractive fusion protein allowing high levels of soluble expression and purification of recombinant protein in E. coli .

Published

2017

42. Discovery of highly reactive peptide tag by ELISA-type screening for specific cysteine conjugation

Author

Shigekazu Tabata, Hirokazu Fuchida, Nobutaka Kurashige, Akio Ojida, and Shohei Uchinomiya

Subjects

Clinical Biochemistry, Pharmaceutical Science, Peptide, Enzyme-Linked Immunosorbent Assay, Protein tag, 010402 general chemistry, Protein labeling, 01 natural sciences, Biochemistry, Maltose-Binding Proteins, Receptors, G-Protein-Coupled, Coordination Complexes, Drug Discovery, Humans, Amino Acid Sequence, Cysteine, Molecular Biology, chemistry.chemical_classification, 010405 organic chemistry, Chemistry, Organic Chemistry, Optical Imaging, Proteins, Isotope-coded affinity tag, Molecular biology, 0104 chemical sciences, Zinc, HEK293 Cells, Molecular Medicine, Peptides, Myc-tag

Abstract

We report the discovery of a highly reactive peptide tag for the specific cysteine conjugation of proteins. Screening of cysteine-containing peptides using ELISA-type screening yielded a 19-amino acid tag (DCPPPDDAADDAADDAADD), named DCP3 tag, which enabled the rapid and selective labeling of the tag-fused protein with a synthetic zinc complex on the surface of living cells.

Published

2017

43. Development of a hexahistidine-3× FLAG-tandem affinity purification method for endogenous protein complexes in Pichia pastoris

Author

Shun-ichi Sekine, Haruhiko Ehara, Noriyuki Suka, Takashi Umehara, Shin Sato, Shigeyuki Yokoyama, Toshiaki Higo, Hideaki Maeda, and Masatoshi Wakamori

Subjects

Recombinant Fusion Proteins, Biochemistry, Article, Chromatography, Affinity, Pichia, Pichia pastoris, Fungal Proteins, Flag sequence, FLAG-tag, Affinity chromatography, Structural Biology, Genetics, Histidine, Tandem affinity purification, Fungal protein, Chromatography, biology, Epitope tagging, General Medicine, biology.organism_classification, Yeast, RNA polymerase, Multiprotein Complexes, Transcription, Myc-tag

Abstract

We developed a method for efficient chromosome tagging in Pichia pastoris, using a useful tandem affinity purification (TAP) tag. The TAP tag, designated and used here as the THF tag, contains a thrombin protease cleavage site for removal of the TAP tag and a hexahistidine sequence (6× His) followed by three copies of the FLAG sequence (3× FLAG) for affinity purification. Using this method, THF-tagged RNA polymerases I, II, and III were successfully purified from P. pastoris. The method also enabled us to purify the tagged RNA polymerase II on a large scale, for its crystallization and preliminary X-ray crystallographic analysis. The method described here will be widely useful for the rapid and large-scale preparation of crystallization grade eukaryotic multi-subunit protein complexes.

Published

2014

44. Intestinal MUC2 Mucin Supramolecular Topology by Packing and Release Resting on D3 Domain Assembly

Author

Philip J.B. Koeck, Elisabeth Thomsson, Malin Bäckström, Hans Hebert, Harriet Nilsson, Daniel Ambort, and Gunnar C. Hansson

Subjects

Colon, Protein Conformation, Size-exclusion chromatography, Green Fluorescent Proteins, Supramolecular chemistry, Mucin 2, CHO Cells, Biology, digestive system, Article, Green fluorescent protein, law.invention, Protein structure, Cricetulus, Imaging, Three-Dimensional, Structural Biology, law, Animals, Humans, Intestinal Mucosa, Molecular Biology, Mucin-2, Mucin, respiratory system, digestive system diseases, Recombinant Proteins, Protein Structure, Tertiary, Crystallography, Microscopy, Electron, Electron microscope, Myc-tag

Abstract

MUC2 is the major gel-forming mucin of the colon forming a protective gel barrier organized into an inner stratified and an outer loose layer. The MUC2 N-terminus (D1-D2-D′D3 domains) has a dual function in building a net-like structure by disulfide-bonded trimerization and packing the MUC2 polymer into an N-terminal concatenated polygonal platform with the C-termini extending perpendicularly by pH- and calcium-dependent interactions. We studied the N-terminal D′D3 domain by producing three recombinant variants, with or without Myc tag and GFP (green fluorescent protein), and analyzed these by gel filtration, electron microscopy and single particle image processing. The three variants were all trimers when analyzed upon denaturing conditions but eluted as hexamers upon gel filtration under native conditions. Studies by electron microscopy and three-dimensional maps revealed cage-like structures with 2- and 3-fold symmetries. The structure of the MUC2 D3 domain confirms that the MUC2 mucin forms branched net-like structures. This suggests that the MUC2 mucin is stored with two N-terminal concatenated ring platforms turned by 180° against each other, implicating that every second unfolded MUC2 net in mature mucus is turned upside down.

Published

2014

45. A Tailor-Made 'Tag-Receptor' Affinity Pair for the Purification of Fusion Proteins

Author

Ana Sofia Pina, Márcia Guilherme, Christopher R. Lowe, Graziella El Khoury, Ricardo J. F. Branco, Cláudia S. M. Fernandes, A. Cecília A. Roque, and Alice S. Pereira

Subjects

Recombinant Fusion Proteins, Green Fluorescent Proteins, Molecular Dynamics Simulation, Ligands, Biochemistry, Chromatography, Affinity, FLAG-tag, Affinity chromatography, Escherichia coli, Amino Acid Sequence, Cloning, Molecular, Molecular Biology, Tandem affinity purification, Binding Sites, Chemistry, Organic Chemistry, Affinity Labels, Isotope-coded affinity tag, Combinatorial chemistry, Fusion protein, Docking (molecular), Molecular Medicine, Affinity electrophoresis, Oligopeptides, Myc-tag

Abstract

A novel affinity "tag-receptor" pair was developed as a generic platform for the purification of fusion proteins. The hexapeptide RKRKRK was selected as the affinity tag and fused to green fluorescent protein (GFP). The DNA fragments were designed, cloned in Pet-21c expression vector and expressed in E. coli host as soluble protein. A solid-phase combinatorial library based on the Ugi reaction was synthesized: 64 affinity ligands displaying complementary functionalities towards the designed tag. The library was screened by affinity chromatography in a 96-well format for binding to the RKRKRK-tagged GFP protein. Lead ligand A7C1 was selected for the purification of RKRKRK fusion proteins. The affinity pair RKRKRK-tagged GFP with A7C1 emerged as a promising solution (Ka of 2.45×10(5) M(-1) ). The specificity of the ligand towards the tag was observed experimentally and theoretically through automated docking and molecular dynamics simulations.

Published

2014

46. Recombinant dengue 2 virus NS3 protein conserves structural antigenic and immunological properties relevant for dengue vaccine design

Author

Emiliana M. Silva, María G. Guzmán, Alienys Izquierdo, Mayra Muné, Ronaldo Mohana-Borges, Ana B. Pérez, Mayling Alvarez, Oney Ortega, Yudira Soto, Angélica García, Rosa Ramírez, and Rosabel Falcón

Subjects

Antigenicity, viruses, Blotting, Western, Fluorescent Antibody Technique, Gene Expression, Dengue Vaccines, Enzyme-Linked Immunosorbent Assay, Viral Nonstructural Proteins, Dengue virus, Antibodies, Viral, medicine.disease_cause, Epitope, Interferon-gamma, Virology, Protein A/G, Escherichia coli, Genetics, medicine, Animals, Cloning, Molecular, Molecular Biology, Dengue vaccine, Mice, Inbred BALB C, Vaccines, Synthetic, NS3, biology, Tumor Necrosis Factor-alpha, Serine Endopeptidases, virus diseases, General Medicine, Dengue Virus, biochemical phenomena, metabolism, and nutrition, Fusion protein, Recombinant Proteins, Interleukin-10, Leukocytes, Mononuclear, biology.protein, Female, RNA Helicases, Myc-tag

Abstract

The NS3 protein is a multifunctional non-structural protein of flaviviruses implicated in the polyprotein processing. The predominance of cytotoxic T cell lymphocytes epitopes on the NS3 protein suggests a protective role of this protein in limiting virus replication. In this work, we studied the antigenicity and immunogenicity of a recombinant NS3 protein of the Dengue virus 2. The full-length NS3 gene was cloned and expressed as a His-tagged fusion protein in Escherichia coli. The pNS3 protein was purified by two chromatography steps. The recombinant NS3 protein was recognized by anti-protease NS3 polyclonal antibody and anti-DENV2 HMAF by Western Blot. This purified protein was able to stimulate the secretion of high levels of gamma interferon and low levels of interleukin-10 and tumor necrosis factor-α in mice splenocytes, suggesting a predominantly Th-1-type T cell response. Immunized BALB/c mice with the purified NS3 protein showed a strong induction of anti-NS3 IgG antibodies, essentially IgG2b, as determined by ELISA. Immunized mice sera with recombinant NS3 protein showed specific recognition of native dengue protein by Western blotting and immunofluorescence techniques. The successfully purified recombinant protein was able to preserv the structural and antigenic determinants of the native dengue protein. The antigenicity shown by the recombinant NS3 protein suggests its possible inclusion into future DENV vaccine preparations.

Published

2014

47. The Biotechnological Applications of Recombinant Single-Domain Antibodies are Optimized by the C-Terminal Fusion to the EPEA Sequence (C Tag)

Author

Ario de Marco, Aurelie Schneider, Anne Beugnet, and Selma Djender

Subjects

lcsh:Immunologic diseases. Allergy, 0106 biological sciences, Immunology, VHH, Protein tag, Biology, immunoprecipitation, 01 natural sciences, antibody screening, tandem affinity purification, law.invention, 03 medical and health sciences, Affinity chromatography, Antigen, law, 010608 biotechnology, Drug Discovery, Immunology and Allergy, Peptide sequence, cytoplasmic antibody expression, nanobody, 030304 developmental biology, Tandem affinity purification, 0303 health sciences, Periplasmic space, Molecular biology, Recombinant DNA, lcsh:RC581-607, Myc-tag

Abstract

We designed a vector for the bacterial expression of recombinant antibodies fused to a double tag composed of 6xHis and the EPEA amino acid sequence. EPEA sequence (C tag) is tightly bound by a commercial antibody when expressed at the C-term end of a polypeptide. The antigen is released in the presence of 2 M MgCl2. Consequently, constructs fused to the 6xHis-C tags can be purified by two successive and orthogonal affinity steps. Single-domain antibodies were produced either in the periplasmic or in the cytoplasmic space of E. coli. Surprisingly, the first affinity purification step performed using the EPEA-binding resin already yielded homogeneous proteins. The presence of the C tag did not interfere with the binding activity of the antibodies, as assessed by FACS and SPR analyses, and the C tag was extremely effective for immunoprecipitating HER2 receptor. Finally, the Alexa488-coupled anti-C tag allowed for simplification of FACS and IF analyses. These results show that a tag of minimal dimensions can be effectively used to improve the applicability of recombinant antibodies as reagents. In our hands, C tag was superior to His-tag in affinity purification and pull-down experiments, and practical in any other standard immune technique.

Published

2014

48. Purification of protein complexes of defined subunit stoichiometry using a set of orthogonal, tag-cleaving proteases

Author

Dirk Görlich, Frey Steffen, and Lidia Goerlich

Subjects

Proteases, medicine.medical_treatment, Protein subunit, SUMO-1 Protein, Clinical Biochemistry, Cleavage (embryo), Biochemistry, Chromatography, Affinity, Controlled subunit stoichiometry, Substrate Specificity, Analytical Chemistry, Tag-removing protease, FLAG-tag, TEV protease, medicine, Histidine, Tandem affinity purification, Chromatography, Protease, Chemistry, On-column cleavage, Organic Chemistry, Protein complex, General Medicine, Recombinant Proteins, Protein Subunits, Multiprotein Complexes, Affinity tag, Molecular Medicine, Peptide Hydrolases, Myc-tag

Abstract

Tag-free proteins or protein complexes represent certainly the most authentic starting points for functional or structural studies. They can be obtained by conventional multi-step chromatography from native or recombinant tag-free sources. Alternatively, they can be expressed and purified using a cleavable N-terminal affinity tag that is subsequently removed by a site-specific protease. Proteolytic tag-removal can also be performed “on-column”. We show here that this not only represents a very efficient workflow, but also drastically improves the purity of the resulting protein preparations. Precondition for effective on-column-cleavage is, however, that the tag-cleaving protease does not bind the stationary phase. We introduce scAtg4 and xlUsp2 as very good and bdSENP1, bdNEDP1 as well as ssNEDP1 as ideal proteases for on-column cleavage at 4 °C. Four of these proteases (bdSENP1, bdNEDP1, scAtg4, xlUsp2) as well as TEV protease display orthogonal, i.e. mutually exclusive cleavage specificities. We combined these features into a streamlined method for the production of highly pure protein complexes: Orthogonal affinity tags and protease recognitions modules are fused to individual subunits. Following co-expression or in-vitro complex assembly, consecutive cycles of affinity capture and proteolytic release then select sequentially for the presence of each orthogonally tagged subunit, yielding protein complexes of well-defined subunit stoichiometry.

Published

2014

49. Challenges and opportunities in the purification of recombinant tagged proteins

Author

Ana C. A. Roque, Christopher R. Lowe, and Ana Sofia Pina

Subjects

Affinity ligands, Strep-tag, Recombinant Fusion Proteins, Bioengineering, Computational biology, Biology, Ligands, Applied Microbiology and Biotechnology, Chromatography, Affinity, Article, law.invention, Mice, Affinity chromatography, FLAG-tag, law, Animals, Humans, Affinity tags, Recombinant proteins, Tandem affinity purification, Chromatography, Fusion protein, Fusion proteins, Recombinant DNA, Target protein, Biotechnology, Myc-tag

Abstract

The purification of recombinant proteins by affinity chromatography is one of the most efficient strategies due to the high recovery yields and purity achieved. However, this is dependent on the availability of specific affinity adsorbents for each particular target protein. The diversity of proteins to be purified augments the complexity and number of specific affinity adsorbents needed, and therefore generic platforms for the purification of recombinant proteins are appealing strategies. This justifies why genetically encoded affinity tags became so popular for recombinant protein purification, as these systems only require specific ligands for the capture of the fusion protein through a pre-defined affinity tag tail. There is a wide range of available affinity pairs “tag-ligand” combining biological or structural affinity ligands with the respective binding tags. This review gives a general overview of the well-established “tag-ligand” systems available for fusion protein purification and also explores current unconventional strategies under development., Highlights • Current and future trends for the purification of recombinant proteins • Comparison of affinity ligands for fusion protein purification • Versatile and unconventional purification strategies for fusion proteins

Published

2014

50. Phosphosite Mapping of HIP-55 Protein in Mammalian Cells

Author

Ningning Sun, Ning Liu, Xiang Gao, and Zijian Li

Subjects

Amino Acid Motifs, Blotting, Western, Molecular Sequence Data, Catalysis, Article, Inorganic Chemistry, src Homology Domains, lcsh:Chemistry, Affinity chromatography, Protein A/G, HSPA2, Humans, Protein phosphorylation, Histidine, Amino Acid Sequence, HIP-55, Physical and Theoretical Chemistry, Molecular Biology, Peptide sequence, lcsh:QH301-705.5, Spectroscopy, Chromatography, High Pressure Liquid, mass spectrometry, Binding Sites, Microscopy, Confocal, biology, phosphorylation, Organic Chemistry, Microfilament Proteins, Protein primary structure, General Medicine, Molecular biology, Computer Science Applications, HEK293 Cells, Biochemistry, lcsh:Biology (General), lcsh:QD1-999, biology.protein, Phosphorylation, Myc-tag

Abstract

In the present study, hematopoietic progenitor kinase 1 (HPK1)-interacting protein of 55 kDa (HIP-55) protein was over-expressed in HEK293 cells, which was genetically attached with 6x His tag. The protein was purified by nickel-charged resin and was then subjected to tryptic digestion. The phosphorylated peptides within the HIP-55 protein were enriched by TiO2 affinity chromatography, followed by mass spectrometry analysis. Fourteen phosphorylation sites along the primary structure of HIP-55 protein were identified, most of which had not been previously reported. Our results indicate that bio-mass spectrometry coupled with manual interpretation can be used to successfully identify the phosphorylation modification in HIP-55 protein in HEK293 cells.

Published

2014