Detection of Soluble CR3 (CD11b/CD18) by Time-Resolved Immunofluorometry

Gitte Krogh Nielsen; Thomas Vorup-Jensen

doi:10.1007/978-1-62703-724-2_30

Detection of Soluble CR₃ (CD11b/CD18) by Time-Resolved Immunofluorometry

Gitte Krogh Nielsen
, Thomas Vorup-Jensen

Research output: Contribution to book/anthology/report/proceeding › Book chapter › Research › peer-review

5 Citations (Scopus)

Abstract

In the cell membrane complement receptor 3 (CR3) consists of one alpha chain (CD11b) and one beta chain (CD18). CR3 participates in many immunological processes, especially those involving cell migration, adhesion, and phagocytosis of complement-opsonized microbes. Recent findings of soluble CR3 in body fluids and in culture supernatant from experiments in vitro point to the involvement of ecto domain shedding as a part of the CR3 biology. To monitor such shedding on a quantitative basis, we have developed time-resolved immunofluorometric assays (TRIFMA) to detect soluble CD11b and CD18 in plasma or serum of either human or murine origin. Compared with most enzyme-linked immunosorbent assays methodologies, TRIFMA possesses prominent advantages, including better dynamic range and reproducibility. These assays may contribute to the understanding of the role of shedding of CR3 and other cell adhesion molecules in human disease and animal models involving inflammation.

Original language	English
Title of host publication	The Complement System : Methods and Protocols
Editors	Mihaela Gadjeva
Number of pages	10
Publisher	Humana Press
Publication date	2014
Pages	355-364
ISBN (Print)	978-1-62703-723-5
ISBN (Electronic)	978-1-62703-724-2
DOIs	https://doi.org/10.1007/978-1-62703-724-2_30 https://doi.org/10.1007/978-1-62703-724-2_30
Publication status	Published - 2014

Series	Methods in Molecular Biology
Volume	1100
ISSN	1064-3745

Keywords

CD11b
CD18
Complement
CR3
Integrin
TRIFMA

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title = "Detection of Soluble CR3 (CD11b/CD18) by Time-Resolved Immunofluorometry",

abstract = "In the cell membrane complement receptor 3 (CR3) consists of one alpha chain (CD11b) and one beta chain (CD18). CR3 participates in many immunological processes, especially those involving cell migration, adhesion, and phagocytosis of complement-opsonized microbes. Recent findings of soluble CR3 in body fluids and in culture supernatant from experiments in vitro point to the involvement of ecto domain shedding as a part of the CR3 biology. To monitor such shedding on a quantitative basis, we have developed time-resolved immunofluorometric assays (TRIFMA) to detect soluble CD11b and CD18 in plasma or serum of either human or murine origin. Compared with most enzyme-linked immunosorbent assays methodologies, TRIFMA possesses prominent advantages, including better dynamic range and reproducibility. These assays may contribute to the understanding of the role of shedding of CR3 and other cell adhesion molecules in human disease and animal models involving inflammation.",

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Detection of Soluble CR₃ (CD11b/CD18) by Time-Resolved Immunofluorometry. / Nielsen, Gitte Krogh; Vorup-Jensen, Thomas.
The Complement System: Methods and Protocols. ed. / Mihaela Gadjeva. Humana Press, 2014. p. 355-364 (Methods in Molecular Biology, Vol. 1100).

Research output: Contribution to book/anthology/report/proceeding › Book chapter › Research › peer-review

TY - CHAP

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AU - Vorup-Jensen, Thomas

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N2 - In the cell membrane complement receptor 3 (CR3) consists of one alpha chain (CD11b) and one beta chain (CD18). CR3 participates in many immunological processes, especially those involving cell migration, adhesion, and phagocytosis of complement-opsonized microbes. Recent findings of soluble CR3 in body fluids and in culture supernatant from experiments in vitro point to the involvement of ecto domain shedding as a part of the CR3 biology. To monitor such shedding on a quantitative basis, we have developed time-resolved immunofluorometric assays (TRIFMA) to detect soluble CD11b and CD18 in plasma or serum of either human or murine origin. Compared with most enzyme-linked immunosorbent assays methodologies, TRIFMA possesses prominent advantages, including better dynamic range and reproducibility. These assays may contribute to the understanding of the role of shedding of CR3 and other cell adhesion molecules in human disease and animal models involving inflammation.

AB - In the cell membrane complement receptor 3 (CR3) consists of one alpha chain (CD11b) and one beta chain (CD18). CR3 participates in many immunological processes, especially those involving cell migration, adhesion, and phagocytosis of complement-opsonized microbes. Recent findings of soluble CR3 in body fluids and in culture supernatant from experiments in vitro point to the involvement of ecto domain shedding as a part of the CR3 biology. To monitor such shedding on a quantitative basis, we have developed time-resolved immunofluorometric assays (TRIFMA) to detect soluble CD11b and CD18 in plasma or serum of either human or murine origin. Compared with most enzyme-linked immunosorbent assays methodologies, TRIFMA possesses prominent advantages, including better dynamic range and reproducibility. These assays may contribute to the understanding of the role of shedding of CR3 and other cell adhesion molecules in human disease and animal models involving inflammation.

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KW - Integrin

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