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Proteostasis

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Cover of 'Proteostasis'

Table of Contents

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    Book Overview
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    Chapter 1 UPS Activation in the Battle Against Aging and Aggregation-Related Diseases: An Extended Review.
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    Chapter 2 Proteostasis
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    Chapter 3 Proteostasis
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    Chapter 4 Immunodepletion and Immunopurification as Approaches for CSN Research.
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    Chapter 5 Proteostasis
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    Chapter 6 Strategies to Detect Endogenous Ubiquitination of a Target Mammalian Protein.
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    Chapter 7 In Vitro Ubiquitination: Self-Ubiquitination, Chain Formation, and Substrate Ubiquitination Assays.
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    Chapter 8 Isolation of the Ubiquitin-Proteome from Tumor Cell Lines and Primary Cells Using TUBEs.
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    Chapter 9 TUBEs-Mass Spectrometry for Identification and Analysis of the Ubiquitin-Proteome.
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    Chapter 10 Isolation of Ubiquitinated Proteins to High Purity from In Vivo Samples.
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    Chapter 11 Method for the Purification of Endogenous Unanchored Polyubiquitin Chains.
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    Chapter 12 Proteostasis
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    Chapter 13 Proteostasis
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    Chapter 14 Monitoring Ubiquitin-Coated Bacteria via Confocal Microscopy
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    Chapter 15 Detection and Analysis of Cell Cycle-Associated APC/C-Mediated Cellular Ubiquitylation In Vitro and In Vivo.
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    Chapter 16 Detection and Analysis of SUMOylation Substrates In Vitro and In Vivo.
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    Chapter 17 Detection of Protein-Protein Interactions and Posttranslational Modifications Using the Proximity Ligation Assay: Application to the Study of the SUMO Pathway.
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    Chapter 18 Dissecting SUMO Dynamics by Mass Spectrometry.
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    Chapter 19 Proteostasis
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    Chapter 20 Proteostasis
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    Chapter 21 Proteostasis
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    Chapter 22 Analysis of Protein Oligomerization by Electrophoresis.
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    Chapter 23 Blot-MS of Carbonylated Proteins: A Tool to Identify Oxidized Proteins.
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    Chapter 24 Proteostasis
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    Chapter 25 A Simple Protocol for High Efficiency Protein Isolation After RNA Isolation from Mouse Thyroid and Other Very Small Tissue Samples.
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    Chapter 26 Monitoring Target Engagement of Deubiquitylating Enzymes Using Activity Probes: Past, Present, and Future.
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    Chapter 27 Proteostasis
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    Chapter 28 Proteostasis
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    Chapter 29 Proteostasis
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    Chapter 30 Using AlphaScreen(®) to Identify Small-Molecule Inhibitors Targeting a Conserved Host-Pathogen Interaction.
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    Chapter 31 Proteostasis
Attention for Chapter 25: A Simple Protocol for High Efficiency Protein Isolation After RNA Isolation from Mouse Thyroid and Other Very Small Tissue Samples.
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Chapter title
A Simple Protocol for High Efficiency Protein Isolation After RNA Isolation from Mouse Thyroid and Other Very Small Tissue Samples.
Chapter number 25
Book title
Proteostasis
Published in
Methods in molecular biology, January 2016
DOI 10.1007/978-1-4939-3756-1_25
Pubmed ID
Book ISBNs
978-1-4939-3754-7, 978-1-4939-3756-1
Authors

Panos G. Ziros Ph.D., Dionysios V. Chartoumpekis M.D., Ph.D., Gerasimos P. Sykiotis M.D., Ph.D., Panos G. Ziros, Dionysios V. Chartoumpekis, Gerasimos P. Sykiotis

Editors

Rune Matthiesen

Abstract

As a dedicated hormone-secreting organ, the thyroid gland possesses a complement of proteostatic systems, including antioxidant, unfolded protein, and autophagic responses. The vast majority of animal investigations of thyroid physiology and, more recently, proteostasis, have utilized as model the rat, rather than the mouse. This is due to the very small size of the thyroid gland in the latter, with a total weight of ~2 mg (~1 mg per thyroid lobe). However, this strategy has limited the utilization of genetic approaches, such as taking advantage of the various transgenic and knockout mouse models. Here, we describe a simple and highly efficient protocol for the simultaneous isolation of mRNA, micro-RNA and 150-200 μg of protein from as little as 1 mg of mouse thyroid tissue, the average weight of one of the two thyroid lobes, thus preserving the other lobe for immunohistochemical or other analyses. While our workflow is similar to other protocols published in the literature and/or proposed by commercial reagent providers, we have introduced a key modification that addresses efficiently the most challenging step of the protein isolation process: the solubilization of the protein pellet after RNA extraction and protein precipitation. We demonstrate the feasibility of our approach and its utility for downstream analyses (including Western blotting) that facilitate the comparative study of proteostatic pathways in the mouse thyroid. We have also successfully applied this protocol on samples from mouse liver, brown and white adipose tissue, as well as from rodent cell lines.

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Mendeley readers

The data shown below were compiled from readership statistics for 10 Mendeley readers of this research output. Click here to see the associated Mendeley record.

Geographical breakdown

Country Count As %
Unknown 10 100%

Demographic breakdown

Readers by professional status Count As %
Student > Ph. D. Student 3 30%
Researcher 2 20%
Professor > Associate Professor 1 10%
Unknown 4 40%
Readers by discipline Count As %
Biochemistry, Genetics and Molecular Biology 4 40%
Computer Science 1 10%
Agricultural and Biological Sciences 1 10%
Medicine and Dentistry 1 10%
Unknown 3 30%