eoe sub articles

EoE Sub Articles

1. Preparation of Genomic DNAs and the Digestion with Restriction Enzyme(s)
<ol>
	<li>Prepare gDNAs from embryonic stem cells (ES cells) using a commercial kit (genomic DNA purification kit) with minor modifications.
	<ol>
		<li>Remove media from the ES cell culture and add 500 &#956;L of nuclei lysis solution, including RNaseA, directly to the wells to lyse the cells. 
		NOTE: The cell lysate can be stored at -80 &#176;C or treated immediately.</li>
		<li>Pipet up and down several times to lyse the cells fully and transfer them to a clean 1.5-mL tube.</li>
		<li>Add one-third of the volume of the protein precipitation solution to the 1.5 mL tube, vortex vigorously for 20 s, chill the samples on ice for 5 min, and then, centrifuge at a force of 2,000 x g for 5 min. Transfer the supernatant to another clean 1.5 mL tube containing an equal volume of isopropanol; gently mix the solution. (Note that white thread-like strands can be seen at this moment.) Centrifuge at a force of 2,000 x g for 1 min; then, discard the supernatant.</li>
		<li>Wash the gDNA pellet with 1 mL of 70% ethanol at room temperature, centrifuge at a force of 2,000 x g for 1 min, aspirate the supernatant carefully, and then, air-dry the gDNA pellet for 3 min.</li>
		<li>Dissolve the gDNAs with 100 &#956;L of DNA rehydration solution and, then, incubate at 65 &#176;C for 1 h or at 4 &#176;C overnight.</li>
		<li>Store the gDNAs at 2&#8211;8 &#176;C.</li>
	</ol>
	</li>
	<li>Digest the gDNAs with predesigned RE Dra I. Set up a 30-&#956;L digestion reaction by mixing 3 &#956;L of 10x buffer for Dra I, 3 &#956;L of Dra I, 10 &#956;g of gDNAs/sample, and H2O up to 30 &#956;L, and incubate at 37 &#176;C overnight.</li>
	<li>Check the completeness of the digestion by DNA gel, analyzing 5 &#956;L of the digested reaction, and then, add the 3 &#956;L of 10x DNA-loading buffer for the subsequent step.</li>
</ol>
2. Southern Blotting
<ol>
	<li>Southern blotting screening
	<ol>
		<li>Separate the digested gDNAs by electrophoresis and transfer them to a membrane.
		<ol>
			<li>Prepare a 1% agarose electrophoresis gel with ethidium bromide (EB), load the digested gDNA samples and a 1 kb ladder, and run the gel with a low voltage (30&#8211;40 V) overnight.</li>
			<li>Take out the gel and take a picture with a DNA gel-imaging system after electrophoresis. Check whether the digested and separated gDNAs display a smear-like image.</li>
			<li>Soak the gel in a tray with 0.2 N HCl solution and shake it gently for 20 min at room temperature.</li>
			<li>Transfer the gel to DNA-denaturing solution and shake it gently for 20 min at room temperature.</li>
			<li>Switch the gel into a DNA-neutralizing solution and shake it gently for 20 min at room temperature. 
			NOTE: The gel is prone to breakage after this step, so it must be handled carefully.</li>
			<li>Use the rapid downward transfer system to transfer the DNAs from the gel to the membrane. Assemble the TurboBlotter and blotting stack according to the instructions provided by the manufacturer. 
			NOTE: 10x or 20x saline-sodium citrate (SSC) solution is used as a transfer buffer. In general, 3 h of transfer is enough to transfer 95% of gDNAs from gel to membrane; however, a longer time of transfer is innocuous.</li>
			<li>Take out the membrane and wash it with 2x SSC for 1 min, absorb the liquid with tissues, and then cross-link the DNA with the membrane using a UV crosslinker. 
			NOTE: The membrane can be stored at 4 &#176;C for one week.</li>
		</ol>
		</li>
	</ol>
	</li>
	<li>Label the DNA probes with radioactivity.
	<ol>
		<li>Purify the probe plasmids using a miniprep kit according to the protocol provided by the manufacturer.</li>
		<li>Release the DNA fragments of the probes from the plasmid vector by EcoR I digestion in a reaction solution including 5 &#181;L of buffer for EcoR I, 2 &#181;L of EcoR I enzyme, 20 &#181;g of plasmid DNA, and H2O up to 50 &#181;L, for 2 h.</li>
		<li>Run a 1% DNA gel for separating the probe DNA fragments from the vector and purify the DNA fragments of the probes with a DNA gel extraction kit according to the protocol provided by the manufacturer.</li>
		<li>Using 1 &#181;L of the DNA solution, measure the DNA concentration of the probe DNA fragments with a spectrophotometer at a wavelength of 260/280 nm.</li>
		<li>Prepare 40-ng of probe DNAs in a 1.5 mL tube with 45 &#181;L of TE buffer, boil for 3 min, spin briefly, and then, place the tube(s) on ice for 2 min.</li>
		<li>Add the heat-denatured probe DNAs to the tube containing ready-to-go DNA-labeling beads (-dCTP), pipet up and down to mix, add 5 &#181;L of [&#945;32P]dCTP, and then, incubate at 37 &#176;C for 15 min.</li>
		<li>Purify the labeled probes by using G-50 microcolumns according to the instructions provided by the manufacturer and, then, measure the radioactivity with a scintillation counter (optional).</li>
	</ol>
	</li>
	<li>Hybridize the membrane(s) with the labeled probes.
	<ol>
		<li>Prehybridize the membrane.
		<ol>
			<li>Prewarm the hybridization solution at 42 &#176;C for 30 min. Mix 20 mL of prewarmed hybridization solution with 200 &#181;g of boiled salmon sperm DNA in a 50-mL tube.</li>
			<li>Place the membrane into the hybridization tube. Add the mixed prehybridization solution to the hybridization tube. Place it into the hybridization oven (set rolling and the temperature at 42 &#176;C) and let the prehybridization proceed for 30 min.</li>
		</ol>
		</li>
		<li>Hybridize the membrane with the labeled probe(s).
		<ol>
			<li>Take out the hybridization tube and pour the prehybridization solution into a 50 mL tube; add the denatured probe (heated at 100 &#176;C for 3 min) from step 2.1.2.7 to this tube and mix gently. 
			NOTE: Reduce any inducing bubbles.</li>
			<li>Return the mixed solution to the hybridization tube and perform the hybridization at 42 &#176;C overnight.</li>
		</ol>
		</li>
	</ol>
	</li>
	<li>Wash the membrane(s) to remove nonhybridized probes.
	<ol>
		<li>Place the membrane(s) into a tray with 1x SSC + 0.1% SDS and shake gently at 55&#8211;60 &#176;C for 10 min.</li>
		<li>Transfer the membrane(s) to a tray with 0.5x SSC + 0.1% SDS and shake gently at 55&#8211;60 &#176;C for 10 min.</li>
		<li>Check the radioactivity on the membrane(s) by using a portable Geiger counter to decide whether a third washing is required.</li>
	</ol>
	</li>
	<li>Expose the radioactivity on the membrane to X-ray films.
	<ol>
		<li>Remove the liquid from the washed membrane(s).</li>
		<li>Enfold the membrane(s) with plastic wrap and fix it/them in the exposure cassette.</li>
		<li>Expose the membrane to two sheets of X-ray film in a dark room.</li>
		<li>Place the exposure cassette at -80 &#176;C overnight or longer.</li>
	</ol>
	</li>
	<li>Develop the films to visualize the results. Evaluate whether a corresponding ES clone is the desired one with the targeted recombination or not, according to the sizes of the DNA bands detected by the probes.</li>
	<li>Rehybridize the same membrane with another probe after stripping off the used probe according to the following procedure: take out the used membrane, wash it 1x with clean H2O, and then, incubate it in striping solution (55% formamide, 2% SSPE, 1% SDS, H2O) at 65 &#176;C with gentle shaking for 1&#8211;2 h.</li>
</ol>

<table><tbody><tr><td>QIAquick Gel Extraction Kit</td><td>QIAGEN</td><td>28704</td><td></td></tr><tr><td>DNA Denaturing Solution</td><td>VWR</td><td>351-013-131</td><td></td></tr><tr><td>DNA Neutralizing Solution</td><td>VWR</td><td>351-014-131</td><td></td></tr><tr><td>EcoR I</td><td>Thermo Scientific</td><td>ER0271</td><td></td></tr><tr><td>Dra I</td><td>Thermo Scientific</td><td>ER0221</td><td></td></tr><tr><td>ProbeQuan G-50 Micro Columns</td><td>GE Healthcare</td><td>28-9034-08</td><td></td></tr><tr><td>Hybrisol I Hybridization Solution</td><td>Millipore</td><td>S4040</td><td></td></tr><tr><td>Ready-To-Go DNA Labeling Beads (-dCTP)</td><td>VWR</td><td>27-9240-01</td><td></td></tr><tr><td>UltraPure SSC, 20x</td><td>Thermo Fisher</td><td>15557036</td><td></td></tr><tr><td>Salmon Sperm DNA Solution</td><td>Thermo Fisher</td><td>15632011</td><td></td></tr><tr><td>Whatman TurboBlotter Transfer System, Large Kits</td><td>Fisher Scientific</td><td>09-301-188</td><td></td></tr><tr><td>[&amp;alpha;32P] dCTP</td><td>PerkinElmer</td><td>NEG013H100UC</td><td></td></tr><tr><td>Kodak X-Ray Film</td><td>Z&amp;amp;Z Medical</td><td>844 5702</td><td></td></tr><tr><td>QIAprep Spin Miniprep Kit</td><td>QIAGEN</td><td>27104</td><td></td></tr><tr><td>Nuclei Lysis Solution</td><td>Promega</td><td>A7941</td><td></td></tr><tr><td>Protein Precipitation Solution</td><td>Promega</td><td>A7951</td><td></td></tr></tbody></table>

southern blotting to detect homologous recombination in the mouse embryonic stem cell genome

Source: Li, J., et al. <a href="https://app.jove.com/v/58467">Identification of Homologous Recombination Events in Mouse Embryonic Stem Cells Using Southern Blotting and Polymerase Chain Reaction.</a> J. Vis. Exp. (2018).
In this video, we describe the Southern blotting technique to identify homologous recombination events in the genome of mouse embryonic stem cells using radiolabeled probes. DNA regions containing homologous recombination events appear as distinct bands when the membrane containing the probe-bound DNA is exposed to X-rays.

Southern Blotting to Detect Homologous Recombination in the Mouse Embryonic Stem Cell Genome

Source: Li, J., et al. Identification of Homologous Recombination Events in Mouse Embryonic Stem Cells Using Southern Blotting and Polymerase Chain ...

Southern blotting involves identifying specific DNA sequences from a complex DNA mix via probe-based detection.
To identify homologous recombination or HR events in mouse embryonic stem cells with Southern blotting, obtain genomic DNA from the cells. Incubate with a restriction enzyme to digest the DNA into smaller fragments.
Load the DNA onto an agarose gel. Perform electrophoresis for size-based fragment separation.
Treat the gel with an acidic solution to remove purine bases, loosening the double-stranded DNA, dsDNA. Add alkaline denaturing solution. The high pH disrupts the hydrogen bonds, denaturing the loosened dsDNA into single-stranded DNA, ssDNA. Incubate with a neutralizing solution to neutralize the gel pH.
Assemble the transfer system using blotting papers, a nylon membrane, and gel stacked on top of the membrane. Perform the transfer. ssDNA transfers from the gel to the membrane via downward capillary action.
Irradiate the membrane with ultraviolet rays, cross-linking and immobilizing the DNA. Place the membrane in a tube containing a hybridization solution. Incubate with rotation, coating the membrane and preventing nonspecific probe binding.
Finally, incubate the membrane with the hybridization buffer containing single-stranded radioactively-labeled probes. The probes bind to specific DNA regions via sequence complementarity.
Wash the membrane, removing unbound probes. Expose the membrane to X-rays. Distinct bands on the membrane distinguish DNA regions containing HR events from control regions.

southern-blotting-to-detect-homologous-recombination-mouse-embryonic

Research

JoVE Encyclopedia of Experiments

Biological Techniques

Blot Techniques

386 次观看. 来源:Li， J. 等人。 使用 Southern 印迹和聚合酶链反应鉴定小鼠胚胎干细胞中的同源重组事件。J. Vis. Exp.（2018 年）。 在本视频中，我们介绍了 Southern 印迹技术，该技术使用放射性标记探针鉴定小鼠胚胎干细胞基因组中的同源重组事件。当包含探针结合 DNA 的膜暴露于 X 射线时，包含同源重组事件的 DNA 区域显示为不同的条带。 

视频: Southern 印迹检测小鼠胚胎干细胞基因组中的同源重组 - 概念

A Method for Measuring RNA N6-methyladenosine Modifications in Cells and Tissues

N6-Methyladenosine (m6A) modifications of RNA are diverse and ubiquitous amongst eukaryotes. They occur in mRNA, rRNA, tRNA, and microRNA. Recent studies have revealed that these reversible RNA modifications affect RNA splicing, translation, degradation, and localization. Multiple physiological processes, like circadian rhythms, stem cell pluripotency, fibrosis, triglyceride metabolism, and obesity are also controlled by m6A modifications. Immunoprecipitation/sequencing, mass spectrometry, and modified northern blotting are some of the methods commonly employed to measure m6A modifications. Herein, we present a northeastern blotting technique for measuring m6A modifications. The current protocol provides good size separation of RNA, better accommodation and standardization for various experimental designs, and clear delineation of m6A modifications in various sources of RNA. While m6A modifications are known to have a crucial impact on human physiology relating to circadian rhythms and obesity, their roles in other (patho)physiological states are unclear. Therefore, investigations on m6A modifications have immense possibility to provide key insights into molecular physiology.

A Method for Measuring RNA N6-methyladenosine Modifications in Cells and Tissues

A modified northern blotting method for measuring N6-methyladenosine (m6A) modifications in RNA is described. The current method can detect modifications in diverse RNAs and controls under various experimental designs.

一种测量方法RNA<em&gt;ñ</em<sup&gt; 6</sup&gt; -methyladenosine细胞和组织修改

N6-Methyladenosine (m6A) modifications of RNA are diverse and ubiquitous amongst eukaryotes. They occur in mRNA, rRNA, tRNA, and microRNA. Recent studies ...

科研

JoVE Journal

生物化学

Modified Terminal Restriction Fragment Analysis for Quantifying Telomere Length Using In-gel Hybridization

There are several different techniques for measuring telomere length, each with their own advantages and disadvantages. The traditional approach, Telomere Restriction Fragment (TRF) analysis, utilizes a DNA hybridization technique whereby genomic DNA samples are digested with restriction enzymes, leaving behind telomere DNA repeats and some sub-telomeric DNA. These are separated by agarose gel electrophoresis, transferred to a filter membrane and hybridized to oligonucleotide probes tagged with either chemiluminescence or radioactivity to visualize telomere restriction fragments. This approach, while requiring a larger quantity of DNA than other techniques such as PCR, can measure the telomere length distribution of a population of cells and allows measurement expressed in absolute kilobases. This manuscript demonstrates a modified DNA hybridization procedure for determining telomere length. Genomic DNA is first digested with restriction enzymes (that do not cut telomeres) and separated by agarose gel electrophoresis. The gel is then dried and the DNA is denatured and hybridized in situ to a radiolabeled oligonucleotide probe. This in situ hybridization avoids loss of telomere DNA and improves signal intensity. Following hybridization, the gels are imaged utilizing phosphor screens and the telomere length is quantified using a graphing program. This procedure was developed by the laboratories of Drs. Woodring Wright and Jerry Shay at the University of Texas Southwestern1,2. Here, we present a detailed description of this procedure, with some modifications.

In this article, a detailed protocol for quantifying telomere length using a modified terminal restriction fragment analysis is discussed that provides fast and efficient direct measurement of telomere length. This technique can be applied to a variety of cell sources of DNA for quantifying telomere length.

使用凝胶内杂交来定量端粒长度的修饰末端限制片段分析

There are several different techniques for measuring telomere length, each with their own advantages and disadvantages. The traditional approach, Telomere ...

癌症研究

Studying Ribonucleotide Incorporation: Strand-specific Detection of Ribonucleotides in the Yeast Genome and Measuring Ribonucleotide-induced Mutagenesis

The presence of ribonucleotides in nuclear DNA has been shown to be a source of genomic instability. The extent of ribonucleotide incorporation can be assessed by alkaline hydrolysis and gel electrophoresis as RNA is highly susceptible to hydrolysis in alkaline conditions. This, in combination with Southern blot analysis can be used to determine the location and strand into which the ribonucleotides have been incorporated. However, this procedure is only semi-quantitative and may not be sensitive enough to detect small changes in ribonucleotide content, although strand-specific Southern blot probing improves the sensitivity. As a measure of one of the most striking biological consequences of ribonucleotides in DNA, spontaneous mutagenesis can be analyzed using a forward mutation assay. Using appropriate reporter genes, rare mutations that results in the loss of function can be selected and overall and specific mutation rates can be measured by combining data from fluctuation experiments with DNA sequencing of the reporter gene. The fluctuation assay is applicable to examine a wide variety of mutagenic processes in specific genetic background or growth conditions.

Ribonucleotides are among the most abundant non-canonical nucleotides incorporated into the genome during eukaryotic nuclear DNA replication. If not properly removed, ribonucleotides can cause DNA damage and mutagenesis. Here, we present two experimental approaches that are used to assess the abundance of ribonucleotide incorporation into DNA and its mutagenic effects.

研究核苷酸合并: 酵母基因组 Ribonucleotides 的链特异检测及核苷酸诱变的检测

The presence of ribonucleotides in nuclear DNA has been shown to be a source of genomic instability. The extent of ribonucleotide incorporation can be ...

Southern Blotting to Detect Homologous Recombination in the Mouse Embryonic Stem Cell Genome

成績單

Southern Blotting to Detect Homologous Recombination in the Mouse Embryonic Stem Cell Genome