We narrowed to 421 results for: sequence

CRISPR Cheat Sheet

• Published: Jan. 27, 2021, 2 p.m.

...: gRNAs: Sequences of RNA that direct the CRISPR system to cut other DNA or RNA sequences. Nucleases...can cut DNA sequences that researchers don’t intend it to. CRISPR cannot cut all sequences. However, prime...Regularly Interspaced Short Palindromic Repeats: Sequences of DNA found in bacteria that allow the bacteria...immune system. Genome Editing: Modifying the DNA sequence of an organism’s genome usually for a research...directed by the gRNAs to cut particular DNA or RNA sequences. Cas9 is a very commonly used CRISPR nuclease....CRISPR: Cut: CRISPR can be used to cut the DNA sequence. With a repair template, CRISPR can be used to...to introduce a functional change in the DNA sequence. Base Editors: Modified versions of CRISPR nucleases...

Plasmids 101: NGS Quality Control for Pooled Libraries

• Published: Oct. 26, 2017, 1:59 p.m.

...quantified, and sent for sequencing. Analyzing your sequencing results If your sequencing is successful, your...next-generation sequencing (NGS). For gRNA libraries, you’ll design primers to create 200-300 bp sequencing products...’s no need to sequence other parts of the plasmid. How will you know if your sequencing results represent...remember when undertaking library amplification and sequencing. Maintain representation of the library during.... Prepare library product for next-generation sequencing Once the DNA has been extracted, the representation... and post-amplification DNA and generates PCR sequencing products from both. These products are then purified...return results in the form of many, many short DNA sequences called reads. Typically they’ll be in a file in...

Plasmid Cloning by PCR

• Published: March 29, 2016, 2:30 p.m.

...8bp) Hybridization Sequence: The region of the primer that binds to the sequence to be amplified (usually...primers for molecular cloning consist of: Leader Sequence: Extra base pairs on the 5' end of the primer ...should use a DNA analysis tool, such as Addgene’s Sequence Analyzer, to allow you to identify which restriction...restriction sites are present in a given sequence. You want to choose enzymes that: Do not cut within your...reverse primer. Next, we need to examine the DNA sequence that we want to amplify and design primers that...Video). Therefore, our Forward Primer will use the sequence 5'-ATGTGGCATATCTCGAAGTAC-3' for the region that...add TAAGCA, resulting in a final Forward Primer sequence of 5'-TAAGCAGAATTCATGTGGCATATCTCGAAGTAC-3'. For...

The PAM Requirement and Expanding CRISPR Beyond SpCas9

• Published: Aug. 20, 2020, 2:30 p.m.

... that (1) the sequence is unique compared to the rest of the genome and (2) the sequence is located just...Protospacer Adjacent Motif (PAM sequence). The 3-5 nucleotide PAM sequence serves as a binding signal for...more PAM sequences While PAM sequences for the commonly used S. pyogenes Cas9 (3'-NGG) are abundant throughout...a target sequence may have high homology elsewhere in the genome. These off-target sequences may be unintentionally...to cleave target DNA sequences located upstream of either NGA or NGC PAM sequences (Kleinstiver et al. ...species PAM sequence may not be characterized Non-SpCas9's bind a variety of PAM sequences, which makes...for Cas9 and this sequence is a strict requirement for Cas9-mediated DNA cleavage. The need for more...

CRISPR 101: Validating Your Genome Edit

• Published: Nov. 3, 2022, 12:15 p.m.

...clones, however, sequence confirmation is still needed to verify the correct sequence was inserted or ...restriction enzyme recognition sequence or generate a new recognition sequence. In these cases, you can screen...edit to mimic what an edited sequence would look like (the 3rd sequencing trace). While it requires a ...technique uses the trace file generated in Sanger sequencing and a simple algorithm to quantify editing efficiency... Fig. 1: Overview of TIDE. The input is sequencing trace files of WT and edited cell lines. Then...amplify the target region of interest. Then Sanger sequence the PCR product of both an unedited population... to the TIDE tool online along with your sgRNA sequence. The TIDE software will generate a graph representing...

Building and Validating Recombinant Antibodies: A Case Study

• Published: April 5, 2022, 1:20 p.m.

...construct by Sanger sequence analysis. But for this research, it was likely that the sequence of the functional...recognition sequence for the restriction enzyme BciVI was present in the aberrant light chain sequence, but ...expression plasmids were DNA sequenced to determine the VH and VL sequence. These plasmids have been deposited...to make the sequences of monoclonal antibodies publicly available. The Neuro Mab Sequencing Initiative ...Initiative uses high-throughput DNA sequencing to determine the VH and VL sequences from the Trimmer lab hybridoma...variable light (VL) and variable heavy (VH) chain sequences. Fusion PCR was performed to create an amplicon...functional VH and VL sequence was not known for each of the mAbs, given the investment it would take to WGS...

Bioinformatics at Addgene

• Published: July 14, 2022, 1:15 p.m.

... us via Sanger sequencing, while more recently we have moved to full plasmid sequencing at our facility...300,000 individual nucleotide sequences. More than half of these sequences were generated by Addgene as...donation of a Illumina MiSeq sequencer enabled us to perform the necessary sequencing on-site, but now we were...needed to transform the raw sequencing data into a complete plasmid sequence that would be ready for our...facility using Illumina MiSeq Next Generation Sequencing (NGS) technology. As our repository continues to ...partnership with Seqera Labs.              DNA sequencing drives our bioinformatics needs       ...pace with our current need to analyze nearly 300 sequences each week. Our internal software was originally...

Simplify Cloning with in vivo Assembly

• Published: Oct. 18, 2018, 12:37 p.m.

...homologous sequences (to 25-30 bp). Tips and tricks for IVA cloning Use a sequence manager A sequence manager...of the vector sequence. Encode homology in the forward primer by adding a short sequence complementary...pieces of linear DNA through short homologous sequences at their termini, and likely functions as a bacterial...assembled in vivo as long as they have homologous sequences at their termini. It doesn’t matter if the DNA...homologous regions can be encoded in the primer sequences. Multiple plasmids can be included in a single...destroy the template, but not newly synthesized sequences, limiting the number of false positive colonies...majority of mistakes are due to incorrect primer sequences! Primers consist of two regions: the 3’ end binds...

Viral Vectors 101: Parts of the AAV Transfer Plasmid

• Published: Aug. 11, 2020, 1:15 p.m.

...plasmid. ITR sequences are 145 bases each and AAV plasmids have two ITR sequences. The DNA sequence between...sites in the ITRs. Regular Sanger sequencing typically fails to sequence through ITRs due to their secondary...now offer Sanger sequencing conditions which can read through this challenging sequence. Transgene The ...first flips the sequence between the first pair of lox sites, and then excise the sequence between the second...an AAV plasmid. Inverted terminal repeat (ITR) sequence Inverted terminal repeats (ITRs) are what makes...be delivered by the AAV. On a plasmid map, its sequence is located between the ITRs. It can be anything... when the transfer plasmid harbors non-coding sequences. Other cis-regulatory elements Next let’s talk...

CRISPR 101: Off-Target Effects

• Published: Feb. 8, 2024, 2:15 p.m.

... other targeted sequencing methods. Candidate site sequencing Sites with high sequence similarity to the... available. Targeted sequencing approaches More targeted alternative sequencing approaches have been ... the gRNA can be sequenced. These sites can be selectively sequenced to determine if there are significant...to a PAM site for DNA cutting to occur. The RNA sequence and PAM site confer specificity of the nuclease...can sometimes localize to unintended sites with sequence similarity to the on-target site. When a CRISPR-Cas...library to thousands of genes and targeting and sequencing millions of cells. For every individual sgRNA...you recover a minimum of 1,000 targeted cells to sequence. In this instance, a 5% off-target frequency is...