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1. ddPCR reactions and droplet generation preparation
<ol>
	<li>Quantify DNA using a fluorometer. 
	NOTE: For the drop-off assay, it is recommended to use a range of 3,000-30,000 haploid genome copies per reaction, which is designed to detect NHEJ events with a HEX-labeling probe that binds to a WT sequence of the targeted cut site and will not anneal (drop-off) if there is a deletion or insertion at the target site, indicating the presence of an NHEJ variant.</li>
	<li>Calculate the copy number using the haploid genome weight and concentration of DNA in the extract. This is done by multiplying the concentration of the extracted DNA by the volume used to obtain the total DNA mass, then dividing it by the haploid genome weight. Ensure that the volume added is between 1-10 &#181;L. Dilute as necessary to be in the recommended haploid genome copy range. 
	NOTE: One Anopheles gambiae haploid genome is estimated to be 0.27 pg per adult mosquito.</li>
	<li>Design primers and probes. Design forward and reverse oligonucleotide primers with a Primer Melting Temperature (Tm) in the range of 55-60 &#176;C that flank the 5&#39;- and 3&#39;-ends of the gRNA target site producing an amplicon of 150-400 bp.
	<ol>
		<li>HEX (Hexachloro-fluorescein)-labeled probe for NHEJ detection: Design an oligonucleotide of ~15-20 bp in length complementary to the target site and add the HEX-probe to the 5&#39;-end and BHQ1 (BLack Hole Quencher 1) to the 3&#39; end. The Tm of the hydrolysis probe should be 3-10 &#176;C higher than the Tm of the primers.</li>
		<li>FAM (6-carboxyfluorescein)-labeled probe for reference WT: Design an oligonucleotide ~15-20 bp in length complementary to a conserved genome site distant (about 25 bp) from the target site and add the FAM-probe to the 5&#39;-end and BHQ1 to the 3&#39; end. The Tm of the hydrolysis probe should be 3-10 &#176;C higher than the Tm of the primers.</li>
	</ol>
	</li>
</ol>
2. PCR reaction preparation
<ol>
	<li>Prepare 25 &#181;L of the ddPCR Sample Mix with the following components: ddPCR supermix for probes (no UTP): 12.5 &#181;L, forward and reverse primers (10 &#181;M): 1 &#181;L each, HEX/FAM probes (10 &#181;M): 0.625 &#181;L each, DNA: 1-5 &#181;L (3,750-37,500 haploid genome copies) and water: up to 25 &#181;L.</li>
	<li>Thoroughly mix the reactions by vortexing or reflux pipetting (up and down) (20x). 
	NOTE: If the reactions are in a 96-well plate, pipette the entire volume up and down 20 times rather than vortexing to avoid bubble formation.</li>
	<li>Briefly centrifuge the samples to settle the mixture at the bottom of the tube or well. 
	NOTE: Ensure the reactions are at room temperature for the droplet generation. Prepare 1x of ddPCR mix for extra/unused wells in each cartridge (each cartridge has 8 wells).</li>
</ol>
3. Droplet generation
<ol>
	<li>Using a 50 &#181;L multichannel pipette, load 20 &#181;L of the ddPCR sample mix into the middle row of the cartridge (Figure 1A, top).</li>
	<li>Load 70 &#181;L of the oil into the bottom row. Load 20 &#181;L of 1x ddPCR supermix into unused wells. 
	NOTE: Do not introduce bubbles.</li>
	<li>Place the gasket touching only the edges, avoiding the center concaved area (Figure 1B).</li>
	<li>Place the plate securely in the droplet generator and close the cover to start the run.</li>
	<li>Using the multichannel pipette, transfer 40 &#181;L of the emersion mix from the top row of the cartridge (Figure 1A, bottom) into the 96-well plate.
	<ol>
		<li>Draw the liquid sample for 3-5 s at a 45-30&#176; angle. Expel the mixture slowly for over 3 s at a 45&#176; angle into the side of the well, allowing it to drip down the side. It is okay to go to the second stop (complete expulsion) of the pipette to expel all the liquid.</li>
	</ol>
	</li>
	<li>Using foil heat seals, seal the plates for 5 s at 180 &#176;C.</li>
</ol>
4. PCR
<ol>
	<li>Place the sealed plate into the thermocycler (Figure 1C) and set the recommended PCR conditions if following the NHEJ Drop-Off guidelines as follows:
	<ol>
		<li>Initial denaturation at 95 &#176;C for 10 min.</li>
		<li>Set 40 cycles of 94 &#176;C for 30 s to denature, 55 &#176;C for 1 min to anneal, and 60 &#176;C for 2 min to extend.</li>
		<li>Hold at 98 &#176;C for 10 min.</li>
		<li>Hold at 4 &#176;C. 
		NOTE: The annealing temperature for specific primers and probe sets may be optimized using a thermal gradient. Use a ramp rate of 2 &#176;C/s for all the steps. PCR conditions should be adjusted depending on each experimental design and set-up.</li>
	</ol>
	</li>
</ol>
5. Droplet reading
<ol>
	<li>Place the plate securely in the droplet reader with well A-1 at the top left (smoothed corner, the other three are edged) (Figure 1D).</li>
	<li>Set up the plate in the program: Designating FAM as the known reference channel and HEX as the unknown one (Figure 2A).</li>
	<li>Run the Droplet reading experiment as direct quantification. After the run finishes, change the Experiment type to Drop-Off (DOF) for the analysis (Figure 2A).</li>
</ol>

<table><tbody><tr><td>&lt;em&gt;&lt;strong&gt;Reagents&lt;/strong&gt;&lt;/em&gt;</td><td></td><td></td><td></td></tr><tr><td>ddPCR Super Mix for Probes (no dUTP)</td><td>Bio-Rad</td><td>1863024</td><td></td></tr><tr><td>EDTA (pH 8.0)</td><td>Invitrogen</td><td>AM9260G</td><td></td></tr><tr><td>PCR-grade Water</td><td></td><td></td><td>Any certified PCR-grade water can be used</td></tr><tr><td>Proteinase K 20 mg/mL</td><td>Thermo Fisher Scientific</td><td>AM2546</td><td></td></tr><tr><td>&lt;em&gt;&lt;strong&gt;Materials&lt;/strong&gt;&lt;/em&gt;</td><td></td><td></td><td></td></tr><tr><td>ddPCR 96-Well Plate</td><td>Bio-Rad</td><td>12001925</td><td></td></tr><tr><td>Droplet Generator DG8 Cartridge and Gaskets</td><td>Bio-Rad</td><td>1864007</td><td></td></tr><tr><td>Droplet Generation Oil for probes</td><td>Bio-Rad</td><td>1863005</td><td></td></tr><tr><td>Fluorescent probes (e.g. FAM/HEX probes)</td><td>Sigma-Aldrich</td><td>N/A</td><td>Probes are experiment specific and can be purchased from any certified seller available.</td></tr><tr><td>Forward and Reverse oligonucleotide primers</td><td>Sigma-Aldrich</td><td>N/A</td><td>Primers are experiment specific and can be purchased from any certified seller available.</td></tr><tr><td>&lt;em&gt;&lt;strong&gt;Equipment&lt;/strong&gt;&lt;/em&gt;</td><td></td><td></td><td></td></tr><tr><td>C1000 Touch Thermal Cycler</td><td>Bio-Rad</td><td>1851148</td><td>Can use other Thermo cycler with gradient function and deep well</td></tr></tbody></table>

digital droplet polymerase chain reaction for indel mutation detection in target genes

Source: Carballar-Lejaraz&#250;, R., et al. <a href="https://app.jove.com/v/62607">Digital-Droplet PCR to Detect Indels Mutations in Genetically Modified Anopheline Mosquito Populations.</a> J. Vis. Exp. (2021).
This video demonstrates the role of digital droplet polymerase chain reaction in identifying indel mutation in a DNA sample. The high precision and sensitivity of ddPCR enable accurate and consistent detection of rare mutations present in a sample, even at low levels. It can identify and quantify indel mutations in different regions of the genome, providing valuable insights into the mechanisms of mutation and the functional consequences of these mutations.&#160;

<img alt="Figure 1" src="/files/ftp_upload/21352/21352_Figure1.jpg" /> 
Figure 1: Experimental setup and procedure. (A) Cartridge preparation for Droplet generation. (Top) Samples are filled in the middle row of the cartridge, while oil is filled in the bottom row. (Bottom) Top row filled with emulsified droplets after droplet generation. (B) Droplet generator with a cartridge filled with sample and covered by a gasket in place. (<st...

Digital Droplet Polymerase Chain Reaction for Indel Mutation Detection in Target Genes

Source: Carballar-Lejaraz&#250;, R., et al. Digital-Droplet PCR to Detect Indels Mutations in Genetically Modified Anopheline Mosquito Populations. J. ...

Digital droplet PCR detects indel mutations &#8212; random insertion or deletion of nucleotides in the DNA. This is achieved by partitioning the sample into tiny droplets and independently amplifying the DNA in each droplet.
To perform ddPCR, take a DNA sample containing wild-type and mutant variations of the target gene. Load the sample mix and oil into distinct compartments of the droplet generator chamber containing the microfluidic channel.
The sample and oil flow rapidly through the narrow channels, emulsify at the junction, and are partitioned into several droplets, each containing a few DNA molecules.
Now, take a PCR plate with the buffer containing forward and reverse primers, dNTPs, thermostable DNA polymerase, and two probes tagged with different fluorophores and quencher molecules. Each probe is specific to a particular type of allele &#8212; wild-type or mutant one.
Transfer the droplets to the PCR plate. Place the plate in a thermocycler, and run the reaction. During denaturation, the DNA strands separate. At annealing temperature, the primers and probes anneal to the template DNA.
The probe with green and orange fluorophores binds to the wild-type and mutant DNA sequence respectively. Later, DNA polymerase extends the primers, cleaving the fluorophore and quencher molecules from the probe, generating a fluorescence signal.
Analyze the amplified product. The droplets showing green fluorescence contain the wild-type DNA sequence, while the orange fluorescence indicates the indel mutation.

digital-droplet-polymerase-chain-reaction-for-indel-mutation

Universidad San Sebastian

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JoVE Encyclopedia of Experiments

Biological Techniques

PCR Techniques

711 Views. Source: Carballar-Lejarazú, R., et al. Digital-Droplet PCR to Detect Indels Mutations in Genetically Modified Anopheline Mosquito Populations. J. Vis. Exp. (2021). This video demonstrates the role of digital droplet polymerase chain reaction in identifying indel mutation in a DNA sample. The high precision and sensitivity of ddPCR enable accurate and consistent detection of rare mutations present in a sample, even at low levels. It can identify and quantify indel mutations in different reg...

Video: Digital Droplet Polymerase Chain Reaction for Indel Mutation Detection in Target Genes - Concept

Efficient Production and Identification of CRISPR/Cas9-generated Gene Knockouts in the Model System Danio rerio

Characterization of the clustered, regularly interspaced, short, palindromic repeat (CRISPR) system of Streptococcus pyogenes has enabled the development of a customizable platform to rapidly generate gene modifications in a wide variety of organisms, including zebrafish. CRISPR-based genome editing uses a single guide RNA (sgRNA) to target a CRISPR-associated (Cas) endonuclease to a genomic DNA (gDNA) target of interest, where the Cas endonuclease generates a double-strand break (DSB). Repair of DSBs by error-prone mechanisms lead to insertions and/or deletions (indels). This can cause frameshift mutations that often introduce a premature stop codon within the coding sequence, thus creating a protein-null allele. CRISPR-based genome engineering requires only a few molecular components and is easily introduced into zebrafish embryos by microinjection. This protocol describes the methods used to generate CRISPR reagents for zebrafish microinjection and to identify fish exhibiting germline transmission of CRISPR-modified genes. These methods include in vitro transcription of sgRNAs, microinjection of CRISPR reagents, identification of indels induced at the target site using a PCR-based method called a heteroduplex mobility assay (HMA), and characterization of the indels using both a low throughput and a powerful next-generation sequencing (NGS)-based approach that can analyze multiple PCR products collected from heterozygous fish. This protocol is streamlined to minimize both the number of fish required and the types of equipment needed to perform the analyses. Furthermore, this protocol is designed to be amenable for use by laboratory personal of all levels of experience including undergraduates, enabling this powerful tool to be economically employed by any research group interested in performing CRISPR-based genomic modification in zebrafish.

Efficient Production and Identification of CRISPR/Cas9-generated Gene Knockouts in the Model System Danio rerio

Targeted genome editing in the model system Danio rerio (zebrafish) has been greatly facilitated by the emergence of CRISPR-based approaches. Herein, we describe a streamlined, robust protocol for generation and identification of CRISPR-derived nonsense alleles that incorporates the heteroduplex mobility assay and identification of mutations using next-generation sequencing.

Characterization of the clustered, regularly interspaced, short, palindromic repeat (CRISPR) system of Streptococcus pyogenes has enabled the development ...

JoVE Journal

Genetics

Studying Wnt Signaling During Patterning of Conducting Airways

Wnt signaling pathways play critical roles during development of the respiratory tract. Defining precise mechanisms of differentiation and morphogenesis controlled by Wnt signaling is required to understand how tissues are patterned during normal development. This knowledge is also critical to determine the etiology of birth defects such as lung hypoplasia and tracheobronchomalacia. Analysis of earliest stages of development of respiratory tract imposes challenges, as the limited amount of tissue prevents the performance of standard protocols better suited for postnatal studies. In this paper, we discuss methodologies to study cell differentiation and proliferation in the respiratory tract. We describe techniques such as whole mount staining, processing of the tissue for confocal microscopy and immunofluorescence in paraffin sections applied to developing tracheal lung. We also discuss methodologies for the study of tracheal mesenchyme differentiation, in particular cartilage formation. Approaches and techniques discussed in the current paper circumvent the limitation of material while working with embryonic tissue, allowing for a better understanding of the patterning process of developing conducting airways.

The use of reporter mice coupled to whole mount and section staining, microscopy and in vivo assays facilitates the analysis of mechanisms underlying the normal patterning of the respiratory tract. Here we describe how these techniques contributed to the analysis of Wnt signaling during tracheal development.

Wnt signaling pathways play critical roles during development of the respiratory tract. Defining precise mechanisms of differentiation and morphogenesis ...

Developmental Biology

Generation of Defined Genomic Modifications Using CRISPR-CAS9 in Human Pluripotent Stem Cells

Human pluripotent stem cells offer a powerful system to study gene function and model specific mutations relevant to disease. The generation of precise heterozygous genetic modifications is challenging due to CRISPR-CAS9 mediated indel formation in the second allele. Here, we demonstrate a protocol to help overcome this difficulty by using two repair templates in which only one expresses the desired sequence change, while both templates contain silent mutations to prevent re-cutting and indel formation. This methodology is most advantageous for gene editing coding regions of DNA to generate isogenic control and mutant human stem cell lines for studying human disease and biology. In addition, optimization of transfection and screening methodologies have been performed to reduce labor and cost of a gene editing experiment. Overall, this protocol is widely applicable to many genome editing projects utilizing the human pluripotent stem cell model.

This protocol provides a method to facilitate the generation of defined heterozygous or homozygous nucleotide changes using CRISPR-CAS9 in human pluripotent stem cells.

Human pluripotent stem cells offer a powerful system to study gene function and model specific mutations relevant to disease. The generation of precise ...

Digital Droplet Polymerase Chain Reaction for Indel Mutation Detection in Target Genes

Transcript

Digital Droplet Polymerase Chain Reaction for Indel Mutation Detection in Target Genes

Efficient Production and Identification of CRISPR/Cas9-generated Gene Knockouts in the Model System Danio rerio

Studying Wnt Signaling During Patterning of Conducting Airways

Generation of Defined Genomic Modifications Using CRISPR-CAS9 in Human Pluripotent Stem Cells