A suitable and effective stepwise oxidative refolding procedure for highly‐cationic tetrameric avidin in nucleic acid free conditions

Kimura, Shuichiro; Imamura, Koreyoshi; Futami, Junichiro

doi:10.1002/btpr.3031

Cited by 3 publications

(4 citation statements)

References 46 publications

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“…The TRIzol extraction procedure quantitatively extracts TCP with complete removal of nucleic acid contamination. After dissolving the extracted proteins in 6 M guanidium hydrochloride (GdnHCl), all cysteine residues were modified via the alkyl disulfide reaction, which enhanced protein solubility by introducing positive charges by TAPS‐sulfonate (Futami et al, 2015; Futami et al, 2017; Kimura et al, 2020; Miyamoto et al, 2022; Murata et al, 2006). Highly water‐soluble TCP was recovered by dialyzing against pure water without any visible precipitates.…”

Section: Resultsmentioning

confidence: 99%

“…The recovered denatured protein precipitates were solubilized in 6 M GdnHCl containing 0.1 M Tris–HCl (pH 8.5) and reduced with 30 mM dithiothreitol for 2 h at 37°C. S ‐cationization of all Cys residues in total cellular proteins was prepared by adding 70 mM [3‐(trimethylammonium)propyl] methanethiosulphonate (TAPS‐sulfonate, Katayama Chemical, Osaka, Japan) and incubating for 1 h at 37°C (Futami et al, 2015; Futami et al, 2017; Kimura et al, 2020; Miyamoto et al, 2022; Murata et al, 2006). Total cellular protein, with or without S ‐cationization, was adjusted to a protein concentration of 3 mg/mL with 6 M GdnHCl and mixed with a 0.1 volume of acetic acid.…”

Section: Methodsmentioning

confidence: 99%

“…To digest nucleic acids, 125 unit/ mL of Benzonase (Merck Millipore, Burlington, MA, USA) were added and incubated for 30 min at 25 C. Nucleic acid-free, fully denatured, and water-soluble total cellular proteins were prepared using TRIzol (Thermo Fisher Scientific, Waltham, MA, USA) according to previously described methods (Futami et al, 2014). The recovered denatured protein precipitates were solubilized in 6 M GdnHCl containing 0.1 M Tris-HCl (pH 8.5) and reduced with 30 mM dithiothreitol for 2 h at 37 C. Scationization of all Cys residues in total cellular proteins was prepared by adding 70 mM [3-(trimethylammonium) propyl] methanethiosulphonate (TAPS-sulfonate, Katayama Chemical, Osaka, Japan) and incubating for 1 h at 37 C (Futami et al, 2015;Futami et al, 2017;Kimura et al, 2020;Miyamoto et al, 2022;Murata et al, 2006). Total cellular protein, with or without Scationization, was adjusted to a protein concentration of 3 mg/mL with 6 M GdnHCl and mixed with a 0.1 volume of acetic acid.…”

Section: Preparation Of Native Cell Lysate and Water-soluble Nucleic ...mentioning

confidence: 99%

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Hydrophobicity and molecular mass‐based separation method for autoantibody discovery from mammalian total cellular proteins

Date,

Miyamoto,

Honjo

et al. 2023

Protein Science

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Serum autoantibody profiles are unique to individuals and reflect the level and history of autoimmunity and tumor immunity. The identification of autoantibody biomarkers is critical for the development of immune monitoring systems for immune‐related disorders. Here, we present a practical method for large‐scale autoantibody discovery using total cellular proteins from cultured mammalian cells. We found that nucleic acid‐free and fully denatured water‐soluble total cellular proteins from mammalian cells were superior, allowing precise separation by reversed‐phase HPLC after preparing a large set of homogeneous total cellular proteins. After separating the proteins based on hydrophobicity, the fractionated samples were subjected to molecular mass analysis using conventional SDS‐PAGE. The resulting two‐dimensional gel electrophoresis was successfully employed for immune blotting and LC–MS/MS analysis. All procedures, including TRIzol‐based total cellular protein extraction, solubilization of denatured proteins, reversed‐phase HPLC separation, and SDS‐PAGE, were highly reproducible and easily scalable. We propose this novel two‐dimensional gel electrophoresis system as an alternative proteomics‐based methodology suitable for large‐scale autoantibody discovery.

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Section: Resultsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Preparation Of Native Cell Lysate and Water-soluble Nucleic ...mentioning

confidence: 99%

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Hydrophobicity and molecular mass‐based separation method for autoantibody discovery from mammalian total cellular proteins

Date,

Miyamoto,

Honjo

et al. 2023

Protein Science

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“…In order to quantitatively evaluate antigen spreading, we designed a multiple S- cationized antigen-immobilized bead array (MUSCAT) assay system ( 33 ). S- cationization techniques are employed as a powerful solubilization tool by conjugation of cationic moieties in sulfhydryl groups in denatured protein ( 34 – 36 ). Full-length and water-soluble S- cationized antigens were covalently immobilized onto Luminex magnetic beads via the activated carboxylic acid of the COOH radical group ( 33 , 37 ).…”

Section: Introductionmentioning

confidence: 99%

Engineering Cancer/Testis Antigens With Reversible S-Cationization to Evaluate Antigen Spreading

et al. 2022

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Serum autoantibody to cancer/testis antigens (CTAs) is a critical biomarker that reflects the antitumor immune response. Quantitative and multiplexed anti-CTA detection arrays can assess the immune status in tumors and monitor therapy-induced antitumor immune reactions. Most full-length recombinant CTA proteins tend to aggregate. Cysteine residue-specific S-cationization techniques facilitate the preparation of water-soluble and full-length CTAs. Combined with Luminex technology, we designed a multiple S-cationized antigen-immobilized bead array (MUSCAT) assay system to evaluate multiple serum antibodies to CTAs. Reducible S-alkyl-disulfide-cationized antigens in cytosolic conditions were employed to develop rabbit polyclonal antibodies as positive controls. These control antibodies sensitively detected immobilized antigens on beads and endogenous antigens in human lung cancer-derived cell lines. Rabbit polyclonal antibodies successfully confirmed the dynamic ranges and quantitative MUSCAT assay results. An immune monitoring study was conducted using the serum samples on an adenovirus−mediated REIC/Dkk−3 gene therapy clinical trial that showed a successful clinical response in metastatic castration-resistant prostate cancer. Autoantibody responses were closely related to clinical outcomes. Notably, upregulation of anti-CTA responses was monitored before tumor regression. Thus, quantitative monitoring of anti-CTA antibody biomarkers can be used to evaluate the cancer-immunity cycle. A quality-certified serum autoantibody monitoring system is a powerful tool for developing and evaluating cancer immunotherapy.

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Removal and monitoring of residual nucleic acids from core streptavidin inclusion bodies for increased refolding yield

Mohamad Alias,

Beng Ong,

Liew

2025

Protein Expression and Purification

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A suitable and effective stepwise oxidative refolding procedure for highly‐cationic tetrameric avidin in nucleic acid free conditions

Cited by 3 publications

References 46 publications

Hydrophobicity and molecular mass‐based separation method for autoantibody discovery from mammalian total cellular proteins

Hydrophobicity and molecular mass‐based separation method for autoantibody discovery from mammalian total cellular proteins

Engineering Cancer/Testis Antigens With Reversible S-Cationization to Evaluate Antigen Spreading

Removal and monitoring of residual nucleic acids from core streptavidin inclusion bodies for increased refolding yield

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