Decellularization and antibody staining of mouse tissues to map native extracellular matrix structures in 3D

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作者
Alejandro E Mayorca-Guiliani
Oliver Willacy
Chris D. Madsen
Maria Rafaeva
Stefanie Elisabeth Heumüller
Felix Bock
Gerhard Sengle
Manuel Koch
Thomas Imhof
Frank Zaucke
Raimund Wagener
Takako Sasaki
Janine T. Erler
Raphael Reuten
机构
[1] University of Copenhagen (UCPH),Biotech Research and Innovation Centre (BRIC)
[2] Lund University,Department of Laboratory Medicine, Division of Translational Cancer Research
[3] Faculty of Medicine and University Hospital Cologne,Center for Biochemistry
[4] University of Cologne,Department of Ophthalmology
[5] Faculty of Medicine and University Hospital Cologne,Center for Molecular Medicine Cologne (CMMC)
[6] University of Cologne,Department of Pediatrics and Adolescent Medicine
[7] University of Cologne,Institute for Dental Research and Oral Musculoskeletal Biology
[8] Faculty of Medicine and University Hospital Cologne,Dr. Rolf M. Schwiete Research Unit for Osteoarthritis
[9] University of Cologne,Department of Biochemistry II, Faculty of Medicine
[10] Faculty of Medicine and University Hospital Cologne,undefined
[11] University of Cologne,undefined
[12] Orthopedic University Hospital Friedrichsheim gGmbH,undefined
[13] Oita University,undefined
来源
Nature Protocols | 2019年 / 14卷
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摘要
The extracellular matrix (ECM) is a major regulator of homeostasis and disease, yet the 3D structure of the ECM remains poorly understood because of limitations in ECM visualization. We recently developed an ECM-specialized method termed in situ decellularization of tissues (ISDoT) to isolate native 3D ECM scaffolds from whole organs in which ECM structure and composition are preserved. Here, we present detailed surgical instructions to facilitate decellularization of 33 different mouse tissues and details of validated antibodies that enable the visualization of 35 mouse ECM proteins. Through mapping of these ECM proteins, the structure of the ECM can be determined and tissue structures visualized in detail. In this study, perfusion decellularization is presented for bones, skeletal muscle, tongue, salivary glands, stomach, duodenum, jejunum/ileum, large intestines, mesentery, liver, gallbladder, pancreas, trachea, bronchi, lungs, kidneys, urinary bladder, ovaries, uterine horn, cervix, adrenal gland, heart, arteries, veins, capillaries, lymph nodes, spleen, peripheral nerves, eye, outer ear, mammary glands, skin, and subcutaneous tissue. Decellularization, immunostaining, and imaging take 4–5 d.
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页码:3395 / 3425
页数:30
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