Name: ビデオ: CRISPRを介した塩基編集ツール:標的塩基置換を誘導するゲノム編集技術 - 概念
Uploaded: 2023-04-30T14:56:11.000+00:00
Duration: 2 min 1 s
Description: 1.4K ビュー. 出典:J.E.他を参照。CRISPR媒介ベースエディターを使用したBRCA1バリアントの機能評価。J. Vis. Exp.(2021年)。 このビデオでは、標的ヌクレオチド置換を誘導するためのCRISPRを介したシトシンベースエディターの概念を説明しています。

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EoE Sub Articles

1. Creation of&#160;BRCA1&#160;variants using CRISPR-mediated base editing tools
NOTE: If HAP1-BE3 cell lines is not used, BE3-encoding plasmid DNA can be co-transfected with&#160;BRCA1-targeting gRNA. Compared to co-transfection of BE3 and gRNA plasmids, transfection of gRNA plasmid to HAP-BE3 cells induce efficient base editing up to 3-fold at target locus in our hands.
<ol>
	<li>Seed 5 x 105&#160;HAP1-BE3 cells (or HAP1 cells in case of co-transfection methods) per well in 24-well plates 1 day prior to transfection. At the time of transfection, culture cells to reach an appropriate density (70%&#8211;80% confluence).</li>
	<li>Transfect&#160;BRCA1-targeting gRNAs using the purchased transfection reagents (Table of Materials) according to the manufacturer&#8217;s protocol. Use 1 &#181;g of&#160;BRCA1-targeting gRNAs (with 1 &#181;g of BE3-encoding plasmid DNA in case of co-transfection methods) to induce C:G to T:A conversion at&#160;BRCA1&#160;target sites. Incubate the cells at 37 &#176;C and subculture every 3&#8211;4 days.</li>
	<li>Harvest the cell pellets 3, 10, and 24 days after transfection to analyze base editing efficiencies (Samples from 3 days after transfection are analyzed regrading as day 0 samples).</li>
	<li>Extract genomic DNA using the genomic DNA purification kit (Table of Materials). 
	NOTE: We recommend optimizing transfection conditions with variable ratio of reagent to DNA. Optimal condition for HAP1 transfection is 4:1 ration of reagent to DNA in our hands.</li>
</ol>

<table><tbody><tr><td>Lipofectamine 2000&amp;nbsp;</td><td>Thermo Fisher Scientific&amp;nbsp;</td><td>11668027</td><td>Transfection reagent</td></tr><tr><td>Opti-MEM&amp;nbsp;</td><td>Gibco&amp;nbsp;</td><td>31985070</td><td>Transfection materials</td></tr><tr><td>FuGENE HD Transfection Reagent&amp;nbsp;</td><td>Promega&amp;nbsp;</td><td>E2311&amp;nbsp;</td><td>Transfection reagent</td></tr><tr><td>Iscove&amp;rsquo;s modified Dulbecco&amp;rsquo;s medium&amp;nbsp;</td><td>Gibco&amp;nbsp;</td><td>12440046</td><td>Medium for HAP1 cells</td></tr><tr><td>lentiCas9-Blast</td><td>&amp;nbsp;Addgene&amp;nbsp;</td><td>52962</td><td>Plasmids DNA for lentiBE3 cloning</td></tr><tr><td>DNeasy Blood &amp;amp; Tissue Kit</td><td>Qiagen</td><td>69504</td><td>Genomic DNA prep. kit</td></tr></tbody></table>

crispr-mediated base editing tools: a genome editing technique to induce targeted base substitution

Source: See, J. E., et al. <a href="https://jove.unicartagenaproxy.elogim.com/v/61557">Functional Assessment of BRCA1 variants using CRISPR-Mediated Base Editors.</a> J. Vis. Exp. (2021).
This video explains the concept of CRISPR-mediated cytosine base editors for inducing targeted nucleotide substitution.

CRISPR-Mediated Base Editing Tools: A Genome Editing Technique to Induce Targeted Base Substitution

Source: See, J. E., et al. Functional Assessment of BRCA1 variants using CRISPR-Mediated Base Editors. J. Vis. Exp. (2021).
This video explains the ...

For CRISPR-mediated genome editing, start with the HAP1-BE3 culture, a haploid cell line with an integrated BE gene encoding a base editor enzyme. To this culture, add lentiviral vectors containing CRISPR-Cas9 plasmid designed for a specific target such as human breast cancer gene, BRCA1.
The lentivirus particle fuses with the host cell membrane, releasing the plasmid, which eventually integrates into the host cell genome to form the CRISPR-Cas9-BE gene segments. These genes generate a BRCA1-targeting gRNA, Cas9 endonuclease, and BE-cytidine deaminase.
The BRCA1-targeting gRNA is an RNA that fuses with Cas9 and directs the complex to the BRCA1 gene locus. Near this gene, locus is a Protospacer Adjacent Motif, or PAM, where BE can stably dock and move upstream to reach its active catalytic region. Here, the BE recognizes a cytidine base and converts it into uridine.
This base substitution mutation triggers Cas9 nuclease to cut the unmodified DNA strand. DNA strand breakage activates repair enzymes that fill in the missing base and convert uracil, a non-DNA base, to thymine. Overall, these processes generate a gene variant.
Now, incubate the cells under physiological conditions and subculture to multiply the gene variant. Extract genomic DNA and sequence it to analyze CRISPR-mediated base editing efficiency.

crispr-mediated-base-editing-tools-genome-editing-technique-to-induce

Universidad de Cartagena UDEC

Research

JoVE Encyclopedia of Experiments

Biological Techniques

Genome Editing Techniques

Gene knock-in

1.4K ビュー. 出典:J.E.他を参照。CRISPR媒介ベースエディターを使用したBRCA1バリアントの機能評価。J. Vis. Exp.(2021年)。 このビデオでは、標的ヌクレオチド置換を誘導するためのCRISPRを介したシトシンベースエディターの概念を説明しています。 

ビデオ: CRISPRを介した塩基編集ツール:標的塩基置換を誘導するゲノム編集技術 - 概念

CRISPR Guide RNA Cloning for Mammalian Systems

The outlined protocol describes streamlined methods for the efficient and cost-effective generation of Cas9-associated guide RNAs. Two alternative strategies for guide RNA (gRNA) cloning are outlined based on the usage of the Type IIS restriction enzyme BsmBI in combination with a set of compatible vectors. Outside of the access to Sanger sequencing services to validate the generated vectors, no special equipment or reagents are required aside from those that are standard to modern molecular biology laboratories. The outlined method is primarily intended for cloning one single gRNA or one paired gRNA-expressing vector at a time. This procedure does not scale well for the generation of libraries containing thousands of gRNAs. For those purposes, alternative sources of oligonucleotide synthesis such as oligo-chip synthesis are recommended. Finally, while this protocol focuses on a set of mammalian vectors, the general strategy is plastic and is applicable to any organism if the appropriate gRNA vector is available.

Here, a simple, efficient, and cost-effective method of sgRNA cloning is outlined.

哺乳類システムのクローン作成 CRISPR ガイド RNA

The outlined protocol describes streamlined methods for the efficient and cost-effective generation of Cas9-associated guide RNAs. Two alternative ...

JoVE Journal

遺伝学

gDNA Enrichment by a Transposase-based Technology for NGS Analysis of the Whole Sequence of BRCA1, BRCA2, and 9 Genes Involved in DNA Damage Repair

The widespread use of Next Generation Sequencing has opened up new avenues for cancer research and diagnosis. NGS will bring huge amounts of new data on cancer, and especially cancer genetics. Current knowledge and future discoveries will make it necessary to study a huge number of genes that could be involved in a genetic predisposition to cancer. In this regard, we developed a Nextera design to study 11 complete genes involved in DNA damage repair. This protocol was developed to safely study 11 genes (ATM, BARD1, BRCA1, BRCA2, BRIP1, CHEK2, PALB2, RAD50, RAD51C, RAD80, and TP53) from promoter to 3&#39;-UTR in 24 patients simultaneously. This protocol, based on transposase technology and gDNA enrichment, gives a great advantage in terms of time for the genetic diagnosis thanks to sample multiplexing. This protocol can be safely used with blood gDNA.

gDNA Enrichment by a Transposase-based Technology for NGS Analysis of the Whole Sequence of BRCA1, BRCA2, and 9 Genes Involved in DNA Damage Repair

gDNA enrichment for NGS sequencing is an easy and powerful tool for the study of constitutional mutations. In this article, we present the procedure to analyse simply the complete sequence of 11 genes involved in DNA damage repair.

の全配列のNGS解析のためのトランスポゼースベースの技術によるgDNAのエンリッチメント<em&gt; BRCA1</em&gt;<em&gt; BRCA2</em&gt;、およびDNA損傷修復に関与する遺伝子9

The widespread use of Next Generation Sequencing has opened up new avenues for cancer research and diagnosis. NGS will bring huge amounts of new data on ...

生物学

Silencing of BRCA2 to Identify Novel BRCA2-regulated Biological Functions in Cultured Human Cells

Silencing of the tumor suppressor protein BRCA2 and its detection by conventional biochemical analyses represent a great technical challenge owing to the large size of the human BRCA2 protein (approximately 390 kDa). We report modifications of standard siRNA transfection and immunoblotting protocols to silence human BRCA2 and detect endogenous BRCA2 protein, respectively, in human epithelial cell lines. Key steps include a high siRNA to transfection reagent ratio and two subsequent rounds of siRNA transfection within the same experiment. Using these and other modifications to the standard protocol we consistently achieve more than 70% silencing of the human BRCA2 gene as judged by immunoblotting analysis with anti-BRCA2 antibodies. In addition, denaturation of the cell lysates at 55 &#176;C instead of the conventional 70-100 &#176;C and other technical optimizations of the immunoblotting procedure allow detection of intact BRCA2 protein even when very low amounts of starting material are available or when BRCA2 protein expression levels are very low. Efficient silencing of BRCA2 in human cells offers a valuable strategy to disrupt BRCA2 function in cells with intact BRCA2, including tumor cells, to examine new molecular pathways and cellular functions that may be affected by pathogenic BRCA2 mutations in tumors. Adaptation of this protocol for efficient silencing and analysis of other &#39;large&#39; proteins like BRCA2 should be readily achievable.

Silencing of BRCA2 to Identify Novel BRCA2-regulated Biological Functions in Cultured Human Cells

Gene silencing by siRNA represents a convenient experimental strategy to analyze BRCA2-dependent biological functions with immediate implications to better understand cancer biology. A method to efficiently silence BRCA2, along with the experimental procedure to detect and quantify changes in BRCA2 protein expression by immunoblotting in human cell lines, is presented.

のサイレンシング<em&gt; BRCA2</em&gt;ヒト培養細胞における新規BRCA2-調節される生物学的機能を同定するために、

Silencing of the tumor suppressor protein BRCA2 and its detection by conventional biochemical analyses represent a great technical challenge owing to the ...

CRISPR-Mediated Base Editing Tools: A Genome Editing Technique to Induce Targeted Base Substitution

記録

CRISPR-Mediated Base Editing Tools: A Genome Editing Technique to Induce Targeted Base Substitution