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Arabidopsis Protocols

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Cover of 'Arabidopsis Protocols'

Table of Contents

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    Book Overview
  2. Altmetric Badge
    Chapter 1 Handling Arabidopsis Plants: Growth, Preservation of Seeds, Transformation, and Genetic Crosses
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    Chapter 2 Using Arabidopsis-Related Model Species (ARMS): Growth, Genetic Transformation, and Comparative Genomics
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    Chapter 3 Growing Arabidopsis In Vitro: Cell Suspensions, In Vitro Culture, and Regeneration
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    Chapter 4 Arabidopsis Database and Stock Resources
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    Chapter 5 Bioinformatic Tools in Arabidopsis Research
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    Chapter 6 Exploiting Natural Variation in Arabidopsis
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    Chapter 7 Grafting in Arabidopsis.
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    Chapter 8 Agrobacterium tumefaciens-Mediated Transient Transformation of Arabidopsis thaliana Leaves
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    Chapter 9 iTILLING: Personalized Mutation Screening
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    Chapter 10 Tailor-Made Mutations in Arabidopsis Using Zinc Finger Nucleases
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    Chapter 11 Arabidopsis Protocols
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    Chapter 12 Generation and Identification of Arabidopsis EMS Mutants
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    Chapter 13 Generation and Characterization of Arabidopsis T-DNA Insertion Mutants
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    Chapter 14 Identification of EMS-Induced Causal Mutations in Arabidopsis thaliana by Next-Generation Sequencing.
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    Chapter 15 Arabidopsis Transformation with Large Bacterial Artificial Chromosomes
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    Chapter 16 Global DNA Methylation Analysis Using Methyl-Sensitive Amplification Polymorphism (MSAP)
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    Chapter 17 Next-Generation Mapping of Genetic Mutations Using Bulk Population Sequencing
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    Chapter 18 Chemical Fingerprinting of Arabidopsis Using Fourier Transform Infrared (FT-IR) Spectroscopic Approaches
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    Chapter 19 A Pipeline for (15)N Metabolic Labeling and Phosphoproteome Analysis in Arabidopsis thaliana.
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    Chapter 20 Gene expression profiling using DNA microarrays.
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    Chapter 21 Forward Chemical Genetic Screening
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    Chapter 22 Highly Reproducible ChIP-on-Chip Analysis to Identify Genome-Wide Protein Binding and Chromatin Status in Arabidopsis thaliana.
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    Chapter 23 Fluorescence Microscopy
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    Chapter 24 Immunocytochemical Fluorescent In Situ Visualization of Proteins In Arabidopsis
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    Chapter 25 High-pressure freezing and freeze substitution of Arabidopsis for electron microscopy.
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    Chapter 26 Applications of Fluorescent Marker Proteins in Plant Cell Biology
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    Chapter 27 Flow Cytometry and Sorting in Arabidopsis
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    Chapter 28 Live Imaging of Arabidopsis Development
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    Chapter 29 Arabidopsis organelle isolation and characterization.
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    Chapter 30 Analysis of Subcellular Metabolite Distributions Within Arabidopsis thaliana Leaf Tissue: A Primer for Subcellular Metabolomics.
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    Chapter 31 Hormone Profiling
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    Chapter 32 Purification of Protein Complexes and Characterization of Protein-Protein Interactions
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    Chapter 33 Protein Fragment Bimolecular Fluorescence Complementation Analyses for the In vivo Study of Protein-Protein Interactions and Cellular Protein Complex Localizations
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    Chapter 34 The Split-Ubiquitin System for the Analysis of Three-Component Interactions
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    Chapter 35 RNA-Binding Protein Immunoprecipitation from Whole-Cell Extracts
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    Chapter 36 High-Throughput Analysis of Protein-DNA Binding Affinity
Attention for Chapter 25: High-pressure freezing and freeze substitution of Arabidopsis for electron microscopy.
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Chapter title
High-pressure freezing and freeze substitution of Arabidopsis for electron microscopy.
Chapter number 25
Book title
Arabidopsis Protocols
Published in
Methods in molecular biology, September 2013
DOI 10.1007/978-1-62703-580-4_25
Pubmed ID
Book ISBNs
978-1-62703-579-8, 978-1-62703-580-4
Authors

Austin JR 2nd, Jotham R. AustinII, Jotham R. Austin

Abstract

The objectives of electron microscopy ultrastructural studies are to examine cellular architecture and relate the cell's structural machinery to dynamic functional roles. This aspiration is difficult to achieve if specimens have not been adequately preserved in a "living state"; hence specimen preparation is of the utmost importance for the success of any electron micrographic study. High-pressure freezing (HPF)/freeze substitution (FS) has long been recognized as the primer technique for the preservation of ultrastructure in biological samples. In most cases a basic HPF/freeze substitution protocol is sufficient to obtain superior ultrastructural preservation and structural contrast, which allows one to use more advanced microscopy techniques such as 3D electron tomography. However, for plant tissues, which have a thick cell wall, large water-filled vacuoles, and air spaces (all of which are detrimental to cryopreservation), these basic HPF/FS protocols often yield undesirable results. In particular, ice crystal artifacts and the staining of membrane systems are often poorly or negatively stained, which make 3D segmentation of a tomogram difficult. To overcome these problems, various aspects of the HPF/FS protocol can be altered, including the cryo-filler(s) used, freeze substitution cocktail, and the resin infiltration process. This chapter will describe these modifications for the preparation of plant tissues for routine electron microscopic studies, immunocytochemistry, and 3D tomographic electron imaging.

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Mendeley readers

The data shown below were compiled from readership statistics for 25 Mendeley readers of this research output. Click here to see the associated Mendeley record.

Geographical breakdown

Country Count As %
Unknown 25 100%

Demographic breakdown

Readers by professional status Count As %
Student > Ph. D. Student 7 28%
Researcher 5 20%
Student > Doctoral Student 2 8%
Student > Bachelor 2 8%
Other 2 8%
Other 5 20%
Unknown 2 8%
Readers by discipline Count As %
Agricultural and Biological Sciences 11 44%
Biochemistry, Genetics and Molecular Biology 5 20%
Chemistry 3 12%
Materials Science 3 12%
Engineering 1 4%
Other 0 0%
Unknown 2 8%
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Attention Score in Context

This research output has an Altmetric Attention Score of 1. This is our high-level measure of the quality and quantity of online attention that it has received. This Attention Score, as well as the ranking and number of research outputs shown below, was calculated when the research output was last mentioned on 11 April 2014.
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#20,228,193
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Outputs of similar age from Methods in molecular biology
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