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CCN Proteins

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Cover of 'CCN Proteins'

Table of Contents

  1. Altmetric Badge
    Book Overview
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    Chapter 1 The CCN Proteins: An Overview.
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    Chapter 2 Gene Expression Analysis of CCN Proteins: Whole-Mount In Situ Hybridization of Ccn2 in Developing Calcified Tissues.
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    Chapter 3 Expression of CCN Genes and Proteins in Human Skin: Methods and Protocols.
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    Chapter 4 Analysis of Expression of CCN Family Genes in Skeletal Tissue-Derived Cells.
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    Chapter 5 Western Blotting Analysis of CCN Proteins in Calcified Tissues.
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    Chapter 6 Immunohistochemical Analysis of CCN Proteins in Calcified Tissues.
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    Chapter 7 Analysis of CCN Expression by Immunofluorescence on Skin Cells, Skin, and Reconstructed Epidermis.
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    Chapter 8 Production of Recombinant CCN2 Protein in Escherichia coli.
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    Chapter 9 Production of Recombinant CCN Proteins by Brevibacillus choshinensis.
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    Chapter 10 Production of Recombinant CCN2 Protein by Mammalian Cells.
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    Chapter 11 In Vitro Transfection with and Expression of CCN Family of Genes.
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    Chapter 12 Preparation of Module-Specific Antibodies Against CCN Family Members.
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    Chapter 13 ELISA of CCN Family Proteins in Body Fluids Including Serum and Plasma.
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    Chapter 14 Analysis of Signaling Pathways Activated by CCN Proteins.
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    Chapter 15 Protocols for Screening for Binding Partners of CCN Proteins: Yeast Two-Hybrid System.
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    Chapter 16 Protocols for Screening Peptide Motifs Binding to CCN Family Proteins.
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    Chapter 17 Evaluation of Molecular Interaction between CCN2 Protein and Its Binding Partners by Surface Plasmon Resonance (SPR).
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    Chapter 18 Promoter Analyses of CCN Genes.
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    Chapter 19 Analysis of Posttranscriptional Regulation of CCN Genes.
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    Chapter 20 Protein Imaging of CCN2 and CCN3 in Living Cells.
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    Chapter 21 Cell Biological Assays for Measuring Chondrogenic Activities of CCN2 Protein.
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    Chapter 22 Cell Biological Assays for Measuring Angiogenic Activities of CCN Proteins.
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    Chapter 23 Cell Biological Assays for Measuring Odontogenic Activities of CCN Proteins.
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    Chapter 24 Separation and Enrichment of Hematopoietic Stem Cells for CCN Studies.
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    Chapter 25 In Vivo Evaluation of Cartilage Regenerative Effects of CCN2 Protein.
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    Chapter 26 Gene Expression Analysis of CCN Protein in Bone Under Mechanical Stress.
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    Chapter 27 The Bone Regeneration Model and Primary Osteoblastic Cell Culture Used in the Analysis of Ccn3 Transgenic and Knockout Mice.
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    Chapter 28 Design and Analysis of CCN Gene Activity Using CCN Knockout Mice Containing LacZ Reporters.
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    Chapter 29 Analysis of CCN4 Function in Osteogenic and Osteoclastic Cells Using Gain and Loss of Function Approaches.
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    Chapter 30 Construction and Analysis of an Allelic Series of Ccn1 Knockin Mice.
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    Chapter 31 Production and Analysis of Conditional KO Mice of CCN2 in Kidney.
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    Chapter 32 Generation and Analysis of Cartilage-Specific CCN2 Overexpression in Transgenic Mice.
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    Chapter 33 Analysis of Transcytosis of CCN2 by Chondrocytes.
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    Chapter 34 CCN2 in Skin Fibrosis.
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    Chapter 35 Studying the CCN Proteins in Fibrosis.
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    Chapter 36 Analysis of Pathological Activities of CCN Proteins in Fibrotic Diseases: Kidney Fibrosis.
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    Chapter 37 Analysis of Pathological Activities of CCN Proteins in Fibrotic Diseases: Liver Fibrosis.
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    Chapter 38 Cellular or Exosomal microRNAs Associated with CCN Gene Expression in Liver Fibrosis.
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    Chapter 39 TGF-β1- and CCN2-Stimulated Sirius Red Assay for Collagen Accumulation in Cultured Cells.
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    Chapter 40 CCN Detection of Cancer Tissues by Immunohistochemistry Staining.
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    Chapter 41 Detection of CCN1 and CCN5 mRNA in Human Cancer Samples Using a Modified In Situ Hybridization Technique.
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    Chapter 42 Analysis of Pathological Activities of CCN Proteins in Bone Metastasis.
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    Chapter 43 Analysis of Pathological Activities of CCN2/CTGF in Muscle Dystrophy.
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    Chapter 44 Method for Analysis of Matrix Degradation by CCN2 Through the MMP/TIMP System.
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    Chapter 45 An Analysis of Pathological Activities of CCN Proteins in Joint Disorders: Mechanical Stretch-Mediated CCN2 Expression in Cultured Meniscus Cells.
  47. Altmetric Badge
    Chapter 46 Analysis of CCN Protein Expression and Activities in Vasoproliferative Retinopathies.
Attention for Chapter 21: Cell Biological Assays for Measuring Chondrogenic Activities of CCN2 Protein.
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Chapter title
Cell Biological Assays for Measuring Chondrogenic Activities of CCN2 Protein.
Chapter number 21
Book title
CCN Proteins
Published in
Methods in molecular biology, January 2017
DOI 10.1007/978-1-4939-6430-7_21
Pubmed ID
Book ISBNs
978-1-4939-6428-4, 978-1-4939-6430-7
Authors

Takashi Nishida D.D.S., Ph.D., Satoshi Kubota, Masaharu Takigawa, Takashi Nishida

Editors

Masaharu Takigawa

Abstract

Growth-plate chondrocytes undergo proliferation, maturation, hypertrophic differentiation, and calcification; and these processes can be reproduced in vitro in a chondrocyte culture system. Using this system, we have shown that CCN family protein 2/connective tissue growth factor (CCN2/CTGF) promotes all stages of proliferation, maturation, hypertrophic differentiation, and calcification, thus suggesting that CCN2 is a multifunctional growth factor for chondrocytes and plays important roles in chondrocyte proliferation and differentiation. In this chapter, we describe how to evaluate CCN2 functions in these processes occurring in cultured chondrocytes. Evaluation strategies for cell proliferation include measuring DNA synthesis by [(3)H]-thymidine incorporation, cellular metabolic activity, and cell number with a hemocytometer. Next, evaluation strategies to assess maturation are analysis of the gene expression of markers of mature chondrocytes, and examination of proteoglycan and collagen synthesis by using radioactive compounds. In addition, cytohistochemical detection of glycosaminoglycans (GAGs), such as chondroitin sulfate, by use of alcian blue and toluidine blue staining is useful to evaluate chondrocyte maturation. These methods can be also used for evaluation of physiological functions of CCN2 in permanent chondrocytes such as articular and auricular chondrocytes, which do not calcify under physiological conditions. Next, evaluation of hypertrophic differentiation is performed by detecting type X collagen, which is specific marker of hypertrophic chondrocytes, and by measuring alkaline phosphatase (ALP) activity. Finally, evaluation of calcification is performed by detecting matrix calcification by use of alizarin red staining and by examining the incorporation of (45)Ca into cartilaginous matrix. These methods would be useful for the evaluation not only of CCN2 but also of its derivatives and other CCN proteins.

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Geographical breakdown

Country Count As %
Unknown 8 100%

Demographic breakdown

Readers by professional status Count As %
Student > Bachelor 3 38%
Professor > Associate Professor 1 13%
Unknown 4 50%
Readers by discipline Count As %
Biochemistry, Genetics and Molecular Biology 1 13%
Agricultural and Biological Sciences 1 13%
Psychology 1 13%
Energy 1 13%
Unknown 4 50%
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