[PDF] Top 20 Resources for the design of CRISPR gene editing experiments

... II CRISPR pro- teins that might possess performance advantages, or to provide altogether new ...new CRISPR systems might necessitate new studies to deter- mine their on- and off-target behavior and ideal ... See full document

... The design of the CRISPR/Cas9 system consists of Cas9 DNA endonuclease and a guide RNA (gRNA) (Figure 1a). Cas9 is fused to the trpC (AN0648) promoter from the Aspergillus nidulans followed by both SV40 ... See full document

... sential for the growth of blood stages (20). We constructed a plas- mid pYC-Pysera1 containing a 46-bp tag DNA (for PCR primers) flanked by two homologous regions of Pysera1 (0.7 kb of the 5=- flanking region and 0.8 kb ... See full document

... the CRISPR-Cas9 site by homology-directed ...genome editing such as creating point mu- tations, adding epitope tags, and introducing stop codons or ...whether CRISPR-Cas9 would facilitate in- sertion ... See full document

... rational design of a combina- tion of sgRNAs can ensure generation of a fragment with two blunt ends, the requirements of sgRNA transcription, together with limited PAM selectivity, will constrain the routine use ... See full document

... growth experiments showed a smaller but still sig- nificant decrease in growth rate (p = ...ase gene following growth in nitrate and urea showed the expected bi-allelic mutation for LM1, M3_9 and M4, ... See full document

... of gene knockdown and deep sequencing technologies that are applicable to a wide range of ...candidate gene approach. The recent discovery of CRISPR/Cas as a means of precise alterations into the ... See full document

... Since Kit w /Kit + and Kit wv /Kit + mice were fertile [17], and as long as one of the two mutation sites is repaired, the Kit w /Kit wv SSCs will restore the differen- tiation ability. We chose WV point for gene ... See full document

... in CRISPR-NHEJ genome editing in mycobacteria. (A) Genome-editing efficiency in ...analysis. Editing efficiency was calculated as the ratio of the number of edited events to the total number of ... See full document

... NFAT5 gene were designed using Broad Institute CRISPRko software [18] (Additional file ...Lenti- CRISPR v2 (Addgene) as a template was PCR-amplified using CRISPR-specific forward primers and a ... See full document

... the design and accuracy of predicting functional sgRNAs for the rat ...in gene activation we observed are due to variations in chromatic state and accessibility in different rat and human ...alternative ... See full document

... for gene editing in ...plasmid-based gene editing system are that any gene can be edited in any isolate in a markerless ...for editing in Candida species other than ...GFP ... See full document

... the CRISPR/Cas9 system provides a simple, sequence-specific platform for genome engineering [14, ...II CRISPR/Cas9 system, which requires a mature CRISPR RNA (crRNA), a trans-acti- vating ... See full document

... II CRISPR adaptive immune system, the RNA-guided agglomerated customarily interspaced short palindrome repeats/CRISPR associated nuclease 9 (CRISPR/Cas9) systems is extracted ...The ... See full document

... a gene, by altering, adding, or taking out pieces of DNA or single base ...a gene from totally different ...the gene for GFP, the glowing green protein from jellyfish, as a biomarker in lots of ... See full document

... Cas9/CRISPR editing solves this issue, existing approaches are inefficient or ...hPSC editing by 2 weeks and required one round of clonal expansion and genotyping rather than two, with similar ... See full document

... SIRT1 is upregulated in KSHV-infected cells SIRT1 is upregulated in several types of human cancer [12, 13, 24]. We examined the expression of SIRT1 in a number of cell types latently infected by KSHV. SIRT1 was ... See full document

... Genetic mapping has become a key element in studying plant disease resis- tance and identifying DNA markers diagnostic of disease resistance. First based on isozymes, the development of more abundant markers progressing ... See full document

... a gene-editing tool to modify donor-extracted T-cells and prepare them to specifically act against tumor cells with enhanced function and durability and least side- ...context, CRISPR technology can ... See full document

... 3.4 CRISPR/Cas9-mediated multiplex gene editing impairs BmNPV replication Next, we wondered if a combination of dual sgRNA or multiple sgRNAs could more effectively inhibit of virus ...one ... See full document