Specific Flow Injection Sandwich Binding Assay for IgG Using Protein A and a Fusion Protein

Publikation: Beitrag in FachzeitschriftArtikelForschungPeer-Review

Autoren

Externe Organisationen

  • Westfälische Wilhelms-Universität Münster (WWU)
  • Medizinische Hochschule Hannover (MHH)
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Details

OriginalspracheEnglisch
Seiten (von - bis)3368-3371
Seitenumfang4
FachzeitschriftAnalytical chemistry
Jahrgang65
Ausgabenummer23
PublikationsstatusVeröffentlicht - 1 Dez. 1993
Extern publiziertJa

Abstract

A sandwich-type flow-injection binding assay for quantitation of various IgG's was developed. The assay is based on the pseudoimmunological reaction between protein A from Staphylococcus aureus and immunoglobulin G from different species. Protein A immobilized on a solid support and a fusion protein of protein A and β-galactosidase from Escherichia coli are used for detection. The fusion protein is produced with a temperature-inducible recombinant E. coli strain. A sandwich is formed by subsequent injection of IgG and fusion protein into the buffer stream flowing through the immobilized protein A column. The amount of enzyme activity bound is proportional to the amount of IgG bound and is measured by pumping a lactose solution as substrate for β-galactosidase through the protein A column. Lactose is converted to glucose and galactose. The detector is an enzyme thermistor that measures the heat evolved in the enzymatic conversion of glucose by coimmobilized glucose oxidase and catalase. The assay takes 16 min at a flow rate of 0.6 mL min-1 with a lower detection limit of 33 pmol per injection of rabbit IgG. The precision of replicate measurements has a standard deviation of 4–5%, and the column can be used for more than 50 cycles.

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Zitieren

Specific Flow Injection Sandwich Binding Assay for IgG Using Protein A and a Fusion Protein. / Brandes, Wiebke; Maschke, Hans Eckhard; Scheper, Thomas.
in: Analytical chemistry, Jahrgang 65, Nr. 23, 01.12.1993, S. 3368-3371.

Publikation: Beitrag in FachzeitschriftArtikelForschungPeer-Review

Brandes W, Maschke HE, Scheper T. Specific Flow Injection Sandwich Binding Assay for IgG Using Protein A and a Fusion Protein. Analytical chemistry. 1993 Dez 1;65(23):3368-3371. doi: 10.1021/ac00071a006
Brandes, Wiebke ; Maschke, Hans Eckhard ; Scheper, Thomas. / Specific Flow Injection Sandwich Binding Assay for IgG Using Protein A and a Fusion Protein. in: Analytical chemistry. 1993 ; Jahrgang 65, Nr. 23. S. 3368-3371.
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T1 - Specific Flow Injection Sandwich Binding Assay for IgG Using Protein A and a Fusion Protein

AU - Brandes, Wiebke

AU - Maschke, Hans Eckhard

AU - Scheper, Thomas

PY - 1993/12/1

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N2 - A sandwich-type flow-injection binding assay for quantitation of various IgG's was developed. The assay is based on the pseudoimmunological reaction between protein A from Staphylococcus aureus and immunoglobulin G from different species. Protein A immobilized on a solid support and a fusion protein of protein A and β-galactosidase from Escherichia coli are used for detection. The fusion protein is produced with a temperature-inducible recombinant E. coli strain. A sandwich is formed by subsequent injection of IgG and fusion protein into the buffer stream flowing through the immobilized protein A column. The amount of enzyme activity bound is proportional to the amount of IgG bound and is measured by pumping a lactose solution as substrate for β-galactosidase through the protein A column. Lactose is converted to glucose and galactose. The detector is an enzyme thermistor that measures the heat evolved in the enzymatic conversion of glucose by coimmobilized glucose oxidase and catalase. The assay takes 16 min at a flow rate of 0.6 mL min-1 with a lower detection limit of 33 pmol per injection of rabbit IgG. The precision of replicate measurements has a standard deviation of 4–5%, and the column can be used for more than 50 cycles.

AB - A sandwich-type flow-injection binding assay for quantitation of various IgG's was developed. The assay is based on the pseudoimmunological reaction between protein A from Staphylococcus aureus and immunoglobulin G from different species. Protein A immobilized on a solid support and a fusion protein of protein A and β-galactosidase from Escherichia coli are used for detection. The fusion protein is produced with a temperature-inducible recombinant E. coli strain. A sandwich is formed by subsequent injection of IgG and fusion protein into the buffer stream flowing through the immobilized protein A column. The amount of enzyme activity bound is proportional to the amount of IgG bound and is measured by pumping a lactose solution as substrate for β-galactosidase through the protein A column. Lactose is converted to glucose and galactose. The detector is an enzyme thermistor that measures the heat evolved in the enzymatic conversion of glucose by coimmobilized glucose oxidase and catalase. The assay takes 16 min at a flow rate of 0.6 mL min-1 with a lower detection limit of 33 pmol per injection of rabbit IgG. The precision of replicate measurements has a standard deviation of 4–5%, and the column can be used for more than 50 cycles.

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