detecting histone modifications in yeast cells with neurodegenerative protein overexpression

Detecting Histone Modifications in Yeast Cells with Neurodegenerative Protein Overexpression

To lyse the cells for western blot analysis, thaw the yeast cell pellets on ice before resuspension in 100 microliters of distilled water. Add 300 microliters of 0.2 molar sodium hydroxide, and 20 microliters of 2-Mercaptoethanol to each cell sample. And resuspend the pellets by pipetting.After a 10-minute incubation on ice, pellet the cells by centrifugation, and resuspend the samples in 100 microliters of loading dye. Then boil the samples for 10 minutes on a heating block. While the samples are being lysed, place two gels in a gel holder, and fill the inner chamber to the top with running buffer and the outside chamber to the two-gel line mark.When the samples are ready, load 15 microliters each cell lysis solution into each well of the 10-well 12% polyacrylamide gel and add 5 microliters of protein ladder to the protein ladder lane well. Run the gel for approximately 45 minutes at 150 volts or until loading dye front reaches the bottom of the gel.While the gel is running, soak two fiber pads per gel in transfer buffer, and one polyvinylidene fluoride or PVDF membrane per gel in methanol. When the gel is ready, rinse membrane and transfer buffer. And place one pre-soaked fiber pad on the bottom of a semi-dry transfer apparatus cell, followed by the PVDF membrane, the gel, and the second pre-soaked fiber pad.Then set the power to 150 milliamps for 1 hour. At the end of the protein transfer, remove the membrane from the transfer apparatus for a brief rinse with distilled water. Place the rinsed membrane protein side up in a small staining box, and cover the membrane with Tris-buffered saline or TBS blocking buffer for a 1 hour incubation at room temperature with gentle rocking.At the end of the blocking incubation, incubate the membrane overnight with an anti-yeast histone and modification specific antibody in TBS at 4 degrees Celsius, and a proper nuclear loading control antibody.The next morning, wash the membrane four times in TBS, supplemented with 0.1% polysorbate 20 for five minutes with rocking at room temperature per wash. After the last wash, incubate the blot with the appropriate secondary antibodies for 1 hour at room temperature, followed by four 5-minute washes in TBST and one five minute wash in TBS alone with rocking.Then image the blot on a fluorescent western blot imaging system for 2 minutes.

detecting-histone-modifications-yeast-cells-with-neurodegenerative

Universidad San Sebastian

Research

JoVE Encyclopedia of Experiments

Neuroscience

Neuropathology

Neurodegenerative Diseases

EoE Sub Articles

eoe sub articles

1. Cell lysis and western blotting to detect histone post-translational modifications<ol><li>Cell lysis<ol style='list-style-type:decimal;'><li>Thaw yeast cell pellets on ice and resuspend cell pellets in 100 &#181;L of dH2O.</li><li>To the cell resuspension, add 300 &#181;L of 0.2 M NaOH and 20 &#181;L of 2-mercaptoethanol. Resuspend by pipetting up and down.</li><li>Incubate cells on ice for 10 min and then centrifuged at 3,200 x&#160;g on a tabletop centrifuge for 30 s at RT. Discard supernatant.</li><li>Resuspend the cell pellet in 100 &#181;L of 1x loading dye and boil for 10 min on a heating block. NOTE:&#160;The recipe for 6x loading dye can be found in the&#160;Table of Materials.</li></ol></li><li>Sodium dodecyl sulfate-polyacrylamide gel electrophoresis and membrane transfer<ol style='list-style-type:decimal;'><li>Prepare the gel chamber by placing two gels in a gel holder filling the inner chamber to the top with running buffer and filling the outside chamber to the two-gel line mark.</li><li>Load 15 &#181;L of sample per well into a 10-well 12% polyacrylamide gel. For the protein ladder lane, load 5 &#181;L.</li><li>Run the gel for approximately 45 minutes at 150 V, or until the loading dye front reaches the bottom of the gel.</li><li>While the gel is running, prepare for membrane transfer by soaking fiber pads (two per gel) in transfer buffer (Table of Materials) and soaking polyvinylidene fluoride (PVDF) membrane in methanol. Rinse the membrane in the transfer buffer before transfer. NOTE: The PVDF membrane should be cut to the size of the gel and use one PVDF membrane for every gel being transferred.</li><li>Assemble, on a semi-dry transfer apparatus cell, a transfer &#8216;sandwich&#8217;: from the bottom electrode, place (1) a presoaked fiber pad, (2) presoaked and rinsed PVDF membrane, (3) gel, and (4) a second presoaked fiber pad. NOTE:&#160;To avoid air bubbles in the transfer &#8216;sandwich, ' gently roll the &#8216;sandwich&#8217; with a serological pipet to force out bubbles. Once the gel has been placed on top of the PDVF membrane, do not move it.</li><li>To carry out protein transfer, set the power pack to 150 mA for 1 h (for one &#8216;sandwich&#8217;).</li></ol></li><li>Detection of histone post-translational modifications (PTMs) with modification-specific antibodies<ol style='list-style-type:decimal;'><li>Remove the membrane from the transfer apparatus. Rinse briefly with dH2O.<ol style='list-style-type:decimal;'><li>Optionally, check the transfer of proteins with Ponceau-S stain by pouring enough Ponceau-S stain to cover the membrane in a small plastic box and incubating at RT with gentle shaking for 30&#8722;60 s. Remove the Ponceau-S stain and rinse with dH2O until the background stain disappears and protein bands are visible to the naked eye. Continue to rinse with dH2O until all stain is removed from the membrane.</li></ol></li><li>Block the membrane by incubating the blot for 1 h at RT with gentle rocking in tris buffered saline (TBS) blocking buffer (Table of Materials) in a small staining box. Use enough blocking buffer to cover the blot. NOTE: Be careful to place the membrane upright in the staining box so that the membrane side on which proteins lie is not facing down.</li><li>Incubate blot in the staining box overnight with a histone modification-specific antibody reactive towards yeast at 4 &#176;C. Dilute the antibody in TBS blocking buffer according to manufacturer specifications. Also include a proper nuclear loading control, such as anti-total H3 raised in a different host species from the modification-specific antibody. For instance, if probing for H3S10ph with an anti-H3S10ph antibody raised in rabbits, use an anti-total H3 antibody raised in mice as a loading control. Repeat this for every blot as necessary. NOTE:&#160;Antibody dilutions can be reused for a total of three times within a month. Store them at 4 &#176;C.</li><li>Wash the membrane 4x in house-made TBS + 0.1% polysorbate 20 (TBST) for 5 min with rocking at RT.</li><li>Incubate blot with fluorescent secondary antibodies at manufacturer-specified dilutions (donkey anti-rabbit 680 and donkey anti-mouse) for 1 h at RT. NOTE:&#160;Fluorescent secondary antibodies must be protected from light during both storage and usage. Carry out incubation in dark plastic boxes or cover with aluminum foil.</li><li>Wash membrane 4x with TBST for 5 min and wash with TBS for 5 min while rocking at RT.</li><li>Visualize blot on a fluorescent Western blot imaging system for 2 min. Visualize the anti-rabbit 680 and anti-mouse 800 secondary antibodies in the 800 nm and 700 nm channels, respectively. NOTE:&#160;Replicates are independently conducted starting from section 1. For appropriate data interpretation in these experiments, it is necessary to verify that the antibody signal response is within the range over which the signal response is linear.</li></ol></li></ol>

<figure class='table' style='width:665pt;'><table class='ck-table-resized'><colgroup><col style='width:20.3%;'><col style='width:16.24%;'><col style='width:16.24%;'><col style='width:47.22%;'></colgroup><tbody><tr><td style='height:62.0pt;width:135pt;'>10x Running Buffer</td><td style='width:108pt;'>&#160;</td><td style='width:108pt;'>&#160;</td><td style='width:314pt;'>Mix: 141.65 g glycine (ThermoFisher BP381-1), 30.3 g Tizma base (Sigma-Aldrich T6066), 10 g sodium dodecyl sulfate (Sigma-Aldrich L3771), and 1 L deionized water, pH 8.8.</td></tr><tr><td style='height:31.0pt;width:135pt;'>12% Polyacrylamide Gels</td><td style='width:108pt;'>BIO-RAD</td><td style='width:108pt;'>456-1041</td><td style='width:314pt;'>&#160;</td></tr><tr><td style='height:15.5pt;width:135pt;'>2-mercaptoethanol</td><td style='width:108pt;'>Sigma-Aldrich</td><td style='width:108pt;'>M3148</td><td style='width:314pt;'>&#160;</td></tr><tr><td style='height:46.5pt;width:135pt;'>Anti-acetyl-Histone H3 (Lys14) Primary Antibody</td><td style='width:108pt;'>MilliporeSigma</td><td style='width:108pt;'>07-353 (Lot No. 2762291)</td><td style='width:314pt;'>Dilution: 1/1000</td></tr><tr><td style='height:46.5pt;width:135pt;'>Anti-acetyl-Histone H4 (Lys16) Primary Antibody</td><td style='width:108pt;'>Abcam</td><td style='width:108pt;'>ab109463 (Lot No. GR187780)</td><td style='width:314pt;'>Dilution: 1/2000</td></tr><tr><td style='height:46.5pt;width:135pt;'>Anti-acetyl-Histone H4 (Lys12) Primary Antibody</td><td style='width:108pt;'>Abcam</td><td style='width:108pt;'>ab46983 (Lot No. GR71882)</td><td style='width:314pt;'>Dilution: 1/5000</td></tr><tr><td style='height:46.5pt;width:135pt;'>Anti-dimethyl-Histone H3 (Lys36) Primary Antibody</td><td style='width:108pt;'>Abcam</td><td style='width:108pt;'>ab9049 (Lot No. GR266894, GR3236147)</td><td style='width:314pt;'>Dilution: 1/1000</td></tr><tr><td style='height:62.0pt;width:135pt;'>Anti-Histone H3 Primary Antibody</td><td style='width:108pt;'>Abcam</td><td style='width:108pt;'>ab24834 (Lot No. GR236539, GR174196, GR3194335)</td><td style='width:314pt;'>Nuclear Loading Control; Dilution: 1/2000</td></tr><tr><td style='height:46.5pt;width:135pt;'>Anti-phospho-Histone H2B (Thr129) Primary Antibody</td><td style='width:108pt;'>Abcam</td><td style='width:108pt;'>ab188292 (Lot No. GR211874)</td><td style='width:314pt;'>Dilution: 1/1000</td></tr><tr><td style='height:62.0pt;width:135pt;'>Anti-phospho-Histone H3 (Ser10) Primary Antibody</td><td style='width:108pt;'>Abcam</td><td style='width:108pt;'>ab5176 (Lot No. GR264582, GR192662, GR3217296)</td><td style='width:314pt;'>Dilution: 1/1000</td></tr><tr><td style='height:15.5pt;width:135pt;'>BioPhotometer D30</td><td style='width:108pt;'>Eppendorf</td><td style='width:108pt;'>6133000010</td><td style='width:314pt;'>&#160;</td></tr><tr><td style='height:31.0pt;width:135pt;'>Centrifuge 5804/5804 R/5810/5810 R</td><td style='width:108pt;'>Eppendorf</td><td style='width:108pt;'>22625501</td><td style='width:314pt;'>&#160;</td></tr><tr><td style='height:62.0pt;width:135pt;'>Donkey Anti-Mouse IRDye 800 CW</td><td style='width:108pt;'>LI-COR</td><td style='width:108pt;'>926-32212 (Lot No. C60301-05, C61116-02, C80108-05)</td><td style='width:314pt;'>Dilution: 1/5000</td></tr><tr><td style='height:77.5pt;width:135pt;'>Donkey Anti-Rabbit IRDye 860 RD</td><td style='width:108pt;'>LI-COR</td><td style='width:108pt;'>926-68073 (Lot No. C60217-06, C70323-06, C70601-05, C80116-07)</td><td style='width:314pt;'>Dilution: 1/2500</td></tr><tr><td style='height:15.5pt;width:135pt;'>Ethanol</td><td style='width:108pt;'>Sigma-Aldrich</td><td style='width:108pt;'>E7023</td><td style='width:314pt;'>&#160;</td></tr><tr><td style='height:31.0pt;width:135pt;'>Extra thick blot paper (filter paper)</td><td style='width:108pt;'>BIO-RAD</td><td style='width:108pt;'>1703968</td><td style='width:314pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:135pt;'>Immobilon-FL Transfer Membranes</td><td style='width:108pt;'>MilliporeSigma</td><td style='width:108pt;'>IPFL00010</td><td style='width:314pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:135pt;'>Loading Dye</td><td style='width:108pt;'>&#160;</td><td style='width:108pt;'>&#160;</td><td style='width:314pt;'>Mix: 1.2 g sodium dodecyl sulfate, 6 mg bromophenol blue (Sigma-Aldrich B8026), 4.7 mL glycerol, 1.2 mL 0.5M Trizma base pH 6.8, 0.93 g DL-Dithiothreitol (Sigma-Aldrich D0632), and 2.1 mL deionized water.</td></tr><tr><td style='height:15.75pt;width:135pt;'>Methanol</td><td style='width:108pt;'>ThermoFisher</td><td style='width:108pt;'>A412-4</td><td style='width:314pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:135pt;'>Mini-PROTEAN Tetra Vertical Electrophoeresis Cell</td><td style='width:108pt;'>BIO-RAD</td><td style='width:108pt;'>1658004</td><td style='width:314pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:135pt;'>Multichannel pipet</td><td style='width:108pt;'>Eppendorf</td><td style='width:108pt;'>2231300045</td><td style='width:314pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:135pt;'>Nuclease Free Water</td><td style='width:108pt;'>Qiagen</td><td style='width:108pt;'>129114</td><td style='width:314pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:135pt;'>Odyssey Fc Imaging System</td><td style='width:108pt;'>LI-COR Biosciences</td><td style='width:108pt;'>2800-03</td><td style='width:314pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:135pt;'>pAG303GAL-a-synuclein-GFP</td><td style='width:108pt;'>Gift from A. Gitler</td><td style='width:108pt;'>&#160;</td><td style='width:314pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:135pt;'>pAG303GAL-ccdB</td><td style='width:108pt;'>Addgene</td><td style='width:108pt;'>14133</td><td style='width:314pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:135pt;'>pAG303Gal-FUS</td><td style='width:108pt;'>Addgene</td><td style='width:108pt;'>29614</td><td style='width:314pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:135pt;'>pAG303GAL-TDP-43</td><td style='width:108pt;'>Gift from A. Gitler</td><td style='width:108pt;'>&#160;</td><td style='width:314pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:135pt;'>Poly(ethylene glycol) (PEG)</td><td style='width:108pt;'>Sigma-Aldrich</td><td style='width:108pt;'>P4338</td><td style='width:314pt;'>Prepare a 50% w/v solution.</td></tr><tr><td style='height:15.75pt;width:135pt;'>Ponceau S Stain</td><td style='width:108pt;'>Sigma-Aldrich</td><td style='width:108pt;'>P3504</td><td style='width:314pt;'>Mix: 0.5 g 0.1% w/w Ponceau S dye, 5 mL 1% v/v acetic acid (Sigma-Aldrich 320099), and 500 mL deionized water.</td></tr><tr><td style='height:15.75pt;width:135pt;'>PowerPac Basic Power Supply</td><td style='width:108pt;'>BIO-RAD</td><td style='width:108pt;'>164-5050</td><td style='width:314pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:135pt;'>Sodium dodecyl sulfate Loading Buffer</td><td style='width:108pt;'>&#160;</td><td style='width:108pt;'>&#160;</td><td style='width:314pt;'>Store at -20 oC. 6X, Mix: 1.2 g sodium dodecyl sulfate, 6 mg bromophenol blue, 0.93 g DL-Dithiothreitol, 2.1 mL deionized water, 4.7 mL glycerol, and 1.2 mL 0.5 M Trizma base, pH 6.8.</td></tr><tr><td style='height:15.75pt;width:135pt;'>Sodium hydroxide</td><td style='width:108pt;'>Sigma-Aldrich</td><td style='width:108pt;'>221465</td><td style='width:314pt;'>Prepare 0.2 M solution.</td></tr><tr><td style='height:15.75pt;width:135pt;'>TBS + 0.1% Tween 20 (TBST)</td><td style='width:108pt;'>&#160;</td><td style='width:108pt;'>&#160;</td><td style='width:314pt;'>Mix: 100 mL 10X TBS, 1 mL Tween 20 (Sigma-Aldrich P7949), and 900 mL deionized water.</td></tr><tr><td style='height:15.75pt;width:135pt;'>TBS Blocking Buffer</td><td style='width:108pt;'>LI-COR</td><td style='width:108pt;'>927-5000</td><td style='width:314pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:135pt;'>Trans-Blot SD Semi-Dry Electrophoretic Transfer Cell</td><td style='width:108pt;'>BIO-RAD</td><td style='width:108pt;'>170-3940</td><td style='width:314pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:135pt;'>Transfer Buffer</td><td style='width:108pt;'>&#160;</td><td style='width:108pt;'>&#160;</td><td style='width:314pt;'>Mix: 22.5 g glycine, 4.84 g Tizma base, 400 mL methanol, 1 g sodium dodecyl sulfate, and 1.6 L deionized water.</td></tr><tr><td style='height:15.75pt;width:135pt;'>Tris-Buffered Saline (TBS)</td><td style='width:108pt;'>&#160;</td><td style='width:108pt;'>&#160;</td><td style='width:314pt;'>10X, 7.6 pH, Solution: Mix 24 g Trizma base, and 88 g sodium chloride (Sigma-Aldrich S7653). Fill to 1 L with deionized water.</td></tr><tr><td style='height:15.75pt;width:135pt;'>WT 303 S. cerevisiae yeast</td><td style='width:108pt;'>Gift from J. Shorter</td><td style='width:108pt;'>&#160;</td><td style='width:314pt;'>&#160;</td></tr></tbody></table></figure>

<a href='https://app-jove-com.bdigitaluss.remotexs.co/v/59104/characterizing-histone-post-translational-modification-alterations'>Source: Bennett, S. A., et al.,&#160;Characterizing Histone Post-translational Modification Alterations in Yeast Neurodegenerative Proteinopathy Models. J. Vis. Exp.&#160;(2019).</a>This video demonstrates the procedure of assessing histone modifications in yeast cells overexpressing neurodegenerative proteins. The steps include cell lysis, centrifugation, electrophoresis, membrane transfer, and antibody-based detection of modified histones.

Source: Bennett, S. A., et al.,&#160;Characterizing Histone Post-translational Modification Alterations in Yeast Neurodegenerative Proteinopathy Models. ...

Begin with a suspension of yeast cells overexpressing proteins linked to neurodegenerative diseases.This overexpressed protein is responsible for modifications in the DNA-packaging proteins or histones with chemical moieties.Add sodium hydroxide and beta-mercaptoethanol and then incubate on ice.&#160;Sodium hydroxide and beta-mercaptoethanol lyse the cells, releasing the intracellular proteins, including histones.Centrifuge the lysate to collect the proteins. Discard the supernatant.Add a loading dye to the protein pellet and heat it to denature them.Load these denatured proteins and a protein marker on the gel and electrophorese to separate them by size.Electrotransfer the proteins onto a membrane, wash, and add a blocking buffer to prevent non-specific binding.Add primary antibodies that specifically bind to modified histones.Wash to remove unbound antibodies and incubate with fluorescent secondary antibodies, which bind to the primary antibodies.A distinct fluorescent band confirms histone modifications, indicating overexpression of neurodegenerative proteins.

15 ビュー. Detecting Histone Modifications in Yeast Cells with Neurodegenerative Protein Overexpression

ビデオ: Detecting Histone Modifications in Yeast Cells with Neurodegenerative Protein Overexpression - 実験

Assays for Validating Histone Acetyltransferase Inhibitors

Lysine acetyltransferases (KATs) catalyze acetylation of lysine residues on histones and other proteins to regulate chromatin dynamics and gene expression. KATs, such as CBP/p300, are under intense investigation as therapeutic targets due to their critical role in tumorigenesis of diverse cancers. The development of novel small molecule inhibitors targeting the histone acetyltransferase (HAT) function of KATs is challenging and requires robust assays that can validate the specificity and potency of potential inhibitors.
This article outlines a pipeline of three methods that provide rigorous in vitro validation for novel HAT inhibitors (HATi). These methods include a test tube HAT assay, Chromatin Hyperacetylation Inhibition (ChHAI) assay, and Chromatin Immunoprecipitation-quantitative PCR (ChIP-qPCR). In the HAT assay, recombinant HATs are incubated with histones in a test tube reaction, allowing for acetylation of specific lysine residues on the histone tails. This reaction can be blocked by a HATi and the relative levels of site-specific histone acetylation can be measured via immunoblotting. Inhibitors identified in the HAT assay need to be confirmed in the cellular environment.
The ChHAI assay uses immunoblotting to screen for novel HATi that attenuate the robust hyperacetylation of histones induced by a histone deacetylase inhibitor (HDACi). The addition of an HDACi is helpful because basal levels of histone acetylation can be difficult to detect via immunoblotting.
The HAT and ChHAI assays measure global changes in histone acetylation, but do not provide information regarding acetylation at specific genomic regions. Therefore, ChIP-qPCR is used to investigate the effects of HATi on histone acetylation levels at gene regulatory elements. This is accomplished through selective immunoprecipitation of histone-DNA complexes and analysis of the purified DNA through qPCR. Together, these three assays allow for the careful validation of the specificity, potency, and mechanism of action of novel HATi.

Inhibitors of histone acetyltransferases (HATs, also known as lysine acetyltransferases), such as CBP/p300, are potential therapeutics for treating cancer. However, rigorous methods for validating these inhibitors are needed. Three in vitro methods for validation include HAT assays with recombinant acetyltransferases, immunoblotting for histone acetylation in cell culture, and ChIP-qPCR.

ヒストンアセチルトランスビセラーゼ阻害剤の検証のためのアッセイ

Lysine acetyltransferases (KATs) catalyze acetylation of lysine residues on histones and other proteins to regulate chromatin dynamics and gene ...

JoVE Journal

がん研究

ヒストンプロテオミクス解析と翻訳後修飾特性評価

Histone Modification Screening using Liquid Chromatography, Trapped Ion Mobility Spectrometry, and Time-Of-Flight Mass Spectrometry

Histone proteins are highly abundant and conserved among eukaryotes and play a large role in gene regulation as a result of structures known as posttranslational modifications (PTMs). Identifying the position and nature of each PTM or pattern of PTMs in reference to external or genetic factors allows this information to be statistically correlated with biological responses such as DNA transcription, replication, or repair. In the present work, a high-throughput analytical protocol for the detection of histone PTMs from biological samples is described. The use of complementary liquid chromatography, trapped ion mobility spectrometry, and time-of-flight mass spectrometry (LC-TIMS-ToF MS/MS) enables the separation and PTM assignment of the most biologically relevant modifications in a single analysis. The described approach takes advantage of recent developments in dependent data acquisition (DDA) using parallel accumulation in the mobility trap, followed by sequential fragmentation and collision-induced dissociation. Histone PTMs are confidently assigned based on their retention time, mobility, and fragmentation pattern.

著者スポットライト:LC-TIMS-ToF、MS/MS、およびPASEFによるヒストンPTM異性体の同定の強化(英語)

An analytical workflow based on liquid chromatography, trapped ion mobility spectrometry, and time-of-flight mass spectrometry (LC-TIMS-ToF MS/MS) for high confidence and highly reproducible "bottom-up" analysis of histone modifications and identification based on principal parameters (retention time [RT], collision cross section [CCS], and accurate mass-to-charge [m/z] ratio).

液体クロマトグラフィー、トラップ型イオンモビリティー分光分析、飛行時間型質量分析を用いたヒストン修飾スクリーニング(英語)

Histone proteins are highly abundant and conserved among eukaryotes and play a large role in gene regulation as a result of structures known as ...

化学

Purification of H3 and H4 Histone Proteins and the Quantification of Acetylated Histone Marks in Cells and Brain Tissue

In all eukaryotic organisms, chromatin, the physiological template of all genetic information, is essential for heredity. Chromatin is subject to an array of diverse posttranslational modifications (PTMs) that mostly occur in the amino termini of histone proteins (i.e., histone tail) and regulate the accessibility and functional state of the underlying DNA. Histone tails extend from the core of the nucleosome and are subject to the addition of acetyl groups by histone acetyltransferases (HATs) and the removal of acetyl groups by histone deacetylases (HDACs) during cellular growth and differentiation. Specific acetylation patterns on lysine (K) residues on histone tails determine a dynamic homeostasis between transcriptionally active or transcriptionally repressed chromatin by (1) influencing the core histone assembly and (2) recruiting synergistic or antagonistic chromatin-associated proteins to the transcription site. The fundamental regulatory mechanism of the complex nature of histone tail PTMs influences the majority of chromatin-templated processes and results in changes in cell maturation and differentiation in both normal and pathological development. The goal of the current report is to provide novices with an efficient method to purify core histone proteins from cells and brain tissue and to reliably quantify acetylation marks on histones H3 and H4.

The purpose of this article is to provide a comprehensive, systematic guide to the efficient purification of histones H3 and H4 and the quantification of acetylated histone residues.

H3 ・ H4 ヒストン蛋白質細胞および脳組織におけるアセチル化ヒストンの定量化の浄化

In all eukaryotic organisms, chromatin, the physiological template of all genetic information, is essential for heredity. Chromatin is subject to an array ...

Detecting Histone Modifications in Yeast Cells with Neurodegenerative Protein Overexpression

記録

Detecting Histone Modifications in Yeast Cells with Neurodegenerative Protein Overexpression