Capillary sodium dodecyl sulfate-DALT electrophoresis with laser-induced fluorescence detection for size-based analysis of proteins in human colon cancer cells

Hu, Shen; Jiang, Jiang; Cook, Lillian M.; Richards, Dawn P.; Horlick, Laura; Wong, Brandon; Dovic̀hi, Norman J.

doi:10.1002/1522-2683(200209)23:18<3136::aid-elps3136>3.0.co;2-s

Cited by 58 publications

(37 citation statements)

References 35 publications

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“…Orange G is a negatively charged marker commonly used in capillary gel electrophoresis applications for determination of protein molecular weight (MW). It has a small MW and migrates faster than protein-SDS molecules through sieving matrices [18]. In this study, OG was chosen in order to simulate the behavior of the negatively charged protein-SDS molecules.…”

Section: Establishment Of the Dynamic Coatmentioning

confidence: 99%

“…The apparent net charge carried out by a protein molecule depends on the isoelectric point (pI) of the protein and pH of the BGE employed [11]. The use of SDS in conjunction with a reducing agent is a commonly used procedure for preparation of protein samples for both conventional and capillary gel electrophoresis [18,19]. This pre-treatment effectively imparts a negative charge on protein molecules proportional to the mass of the protein (&1.4 g SDS/g protein).…”

Section: Introductionmentioning

confidence: 99%

“…This pre-treatment effectively imparts a negative charge on protein molecules proportional to the mass of the protein (&1.4 g SDS/g protein). Protein-SDS complexes migrate at the same speed under the effect of an applied electric field [18][19][20][21].…”

Section: Introductionmentioning

confidence: 99%

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CZE with On-line Micellar Sample Stacking for Determination of Protein Concentration of Biopharmaceuticals

et al. 2011

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A capillary zone electrophoresis total protein assay was developed and validated in polyethylene oxide (PEO) dynamically coated capillaries. On-line large-volume sample stacking was employed. Protein samples were denatured using SDS and then injected into PEO-filled capillaries. Such treatment enabled injection of a sample volume of &8% of the total capillary volume and stacking of protein-SDS molecules at the interface between the sample plug and the PEO plug. Results showed that SDS enhanced the sensitivity not only by protein denaturation but also by forming micelles, in which protein-SDS partitioned. Sensitivity of the method was further enhanced through using capillaries with (tenfold) extended detection pathlength. Such strategies resulted in a limit of detection of 0.26 lg mL -1 (3.64 nM BSA). A linear relationship between protein concentration and integrated peak area was obtained over a wide concentration range (8.49-135.87 lg mL -1 -R 2 = 0.995). The method is particularly useful for determination of total protein concentration in chromatography fractions. It overcomes low UV absorptivity of proteins, presence of UV absorbing additives and high salt content. Contrary to conventional methods for determination of protein concentration, this method does not involve an interaction with a dye. Thus, variations due to differences in surface properties among proteins or due to differences in posttranslational modifications of the same protein are eliminated. The protocol was successfully applied for the determination of the concentration of a biopharmaceutical protein rhMBP in chromatography fractions. This protein has been previously produced in milk of transgenic cows and several charge isoforms were detected.

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Section: Establishment Of the Dynamic Coatmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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CZE with On-line Micellar Sample Stacking for Determination of Protein Concentration of Biopharmaceuticals

et al. 2011

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“…Our group reported a series of papers applying CSE methods for highly sensitive protein analysis for cell homogenates and single cells using 3-(2-furoyl)quinoline-2-carboxaldehyde (FQ), a fluorogenic reagent (31)(32)(33). The labeled proteins were separated in a replaceable polymer sieving matrix such as PEO or pullulan and then detected using an ultrasensitive sheath-flow laser-induced fluorescence detector.…”

Section: Proteins and Peptidesmentioning

confidence: 99%

Capillary Electrophoresis for the Analysis of Biopolymers

Quigley

Dovic̀hi

2004

Anal. Chem.

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suppress EOF. However, the conductivity of these buffers is relatively high, resulting in high current, excessive Joule heating, and the electrolysis of water causing bubble formation during the separation. These phenomena may lead to peak broadening, loss Table 1. Separation of Proteins by CE a mode b sample c capillary buffer detection d LOD ref CZE human immunoglobin G uncoated 15-100 mM H3PO4, 20 mM borate, various amounts of ACN, PEG, Triton-X, and SDS 3 CZE model proteins; Lys, Cyt, Chy, Try coated and uncaoted 40 mM acetate, pH 4.5 UV 4 CZE human serum; globulin isoforms, HAS, transferrin uncoated proprietary reagent set UV 5 CZE human serum; transferrin isoforms proprietary dynamic double coating unreported Tris/borate concn, pH 10 UV 6 CZE model proteins; RibA, BSA, ADH, Lys PB dynamic coating 2 mM PB 5mM Tris LIF amol 7

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“…Further complicating attempts to label proteins by fluorescent tags is the requirement that both protein and dye are present in higher concentrations for the reaction to proceed, 4 although exceptions have been reported. 5 Non-covalent fluorescent labelling and quenching of proteins has been an important method in the study of protein folding. 6 Non-covalent labels used thus far include indocyanine green, 7 squarylium dyes, 8 NanoOrange, 9 and the SYPRO series of dyes.…”

Section: Introductionmentioning

confidence: 99%

In-Gel Staining of Proteins in Native Poly Acryl Amide Gel Electrophoresis Using Tetrakis(4-sulfonato phenyl)porphyrin

et al. 2011

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Protein identification in polyacrylamide gel electrophoresis (PAGE) requires post-electrophoretic steps like fixing, staining and destaining of the gel, which are time-consuming and cumbersome. We have developed a method for direct visualization of protein bands in PAGE using tetrakis(4-sulfonato phenyl)porphyrin (TPPS) as a dye without the need for any post electrophoretic steps, where separation and recovery of enzymes become much easier for further analysis. Activity staining was done to prove that the biochemical activity of the enzymes was preserved after electrophoresis.

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Capillary sodium dodecyl sulfate-DALT electrophoresis with laser-induced fluorescence detection for size-based analysis of proteins in human colon cancer cells

Cited by 58 publications

References 35 publications

CZE with On-line Micellar Sample Stacking for Determination of Protein Concentration of Biopharmaceuticals

CZE with On-line Micellar Sample Stacking for Determination of Protein Concentration of Biopharmaceuticals

Capillary Electrophoresis for the Analysis of Biopolymers

In-Gel Staining of Proteins in Native Poly Acryl Amide Gel Electrophoresis Using Tetrakis(4-sulfonato phenyl)porphyrin

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