LentiCRISPRv2 and lentiGuide-Puro: lentiviral CRISPR/Cas9 and single guide RNA CRISPR (C lustered R egularly I nterspaced S hort P alindromic R epeats) is a microbial nuclea system involved in defen against invading phages and plasmids. CRISPR loci in microbial hosts contain a combination of CRISPR-associated (Cas) genes as well as non-coding RNA elements capable of programming the specificity of the CRISPR-mediated nucleic acid cleavage. Lentiviral CRISPR/Cas can infect a broad variety of mammalian cells by co-expressing a mammalian codon-optimized Cas9 nuclea along with a single guide RNA (sgRNA) to facilitate genome editing (Shalem*, Sanjana*, et al., Science 2014). Protocols for cloning into the lentiviral transfer plasmid and general considerations for producing lentivirus are described below. Separate protocols are available for amplifying the genome-scale CRISPR knock-out (GeCKO) libraries. This protocol is for creating individual lentiviral CRISPR plasmids targeting a single genomic locus.
lentiCRISPRv2 (one vector system): This plasmid contains two expression casttes, hSpCas9 and the chimeric guide RNA. The vector can be digested using BsmB I, and a pair of annealed oligos can be cloned into the single guide RNA scaffold. The oligos are designed bad on the target site quenc
西瓜营养e (20bp) and needs to be flanked on the 3' end by a 3bp NGG PAM quence, as shown on the next page.
lentiGuide-Puro (two vector system): This plasmid expresd only the chimeric guide RNA. It does not contain Cas9. Plea u lentiCas9-Blast (a parate lentiviral construct that delivers hSpCas9 and blasticidin resistance) to first integrate Cas9 into your cell line. The lentiGuide-Puro vector can be digested using BsmB I, and a pair of annealed oligos can be cloned into the single guide RNA scaffold. The oligos are designed bad on the target site quence (20bp) and needs to be flanked on the 3' end by a 3bp NGG PAM quence, as shown on the next page.什么茶叶去火
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Which vector to u: lentiCRISPRv2 is identical to the original lentiCRISPRv1 but produces nearly 10X higher titer virus. lentiGuide-Puro produces >100X higher titer virus over lentiCRISPRv1 and sh
ould be ud in cell lines where Cas9 has already been integrated in (e.g. using the parate lentiCas9-Blast lentivirus). For applications where Cas9 cannot first be introduced (e.g. primary cells), lentiCRISPRv2 is recommended. After transduction, u puromycin to lect for cells with lentiCRISPRv2 or lentiGuide-Puro.
大班诗歌《我长大了》Lentiviral production: Before starting any lentiviral work, plea ensure compliance with your Environmental Health and Safety office and government/organization/university. Briefly, to make lentivirus, a transfer plasmid (e.g. lentiCRISPRv2 or lentiGuide-Puro) must be co-transfected into HEK293(F)T cells with the packaging plasmids pVSVg (AddGene 8454) and psPAX2 (AddGene 12260). As a positive control for viral production, we often u a CMV-EGFP lentiviral transfer plasmid (eg. AddGene 19319).
Target design notes and online resources: For application of Cas9 for site-specific genome editing in eukaryotic cells and organisms, we have computationally identified suitable target sites for the S. pyogenes Cas9 and calculated most likely off-targets within the genome. Plea visit to access the Cas9 target design tools. Complete plasmid quences, protocols, a discussion forum and additional information can be found at the Zhang Lab GeCKO website: /gecko/ . Citation: Plea reference the followin
g publications for the u of this material.
Improved lentiviral vectors and genome-wide libraries for CRISPR screening. Sanjana NE*, Shalem O*, Zhang F. Nature Methods (2014).
Genome-scale CRISPR-Cas9 knockout screening in human cells. Shalem O*, Sanjana NE*, Hartenian E, Shi X, Scott DA, Mikkeln T, Heckl D, Ebert BL, Root DE, Doench JG, Zhang F (2014). Science, 343, 83-7. DOI: 10.1126/science.1247005
Target Guide Sequence Cloning Protocol
In order to clone the target quence into the lentiCRISPRv2 or lentiGuide-Puro backbone, synthesize two oligos of the following form. All plasmids have the same overhangs after BsmBI digestion and the same oligos can be ud for cloning into lentiCRISPRv2, lentiGuide-Puro or lentiCRISPRv1.
Example oligo design
: Note that the NGG PAM is not included in the designed oligos. Oligonucleotide ordering tips : Standard de-salted oligos (usually the most inexpensive synthesis) are sufficient for
cloning. If not already resuspended, dilute each oligo to 100 µM in sterile water or TE.
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Lentiviral vector digestion, oligo annealing and cloning into digested vector:
1. Digest and dephosphorylate 5ug of the lentiviral CRISPR plasmid with BsmB I for 30 min at 37C: 5 ug lentiCRISPRv2 or lentiGuide-Puro 3 ul FastDigest BsmB I (Fermentas) 3 ul FastAP (Fermentas) 6 ul 10X FastDigest Buffer 0.6 ul 100 mM DTT (freshly prepared) X ul ddH 2O 60 ul total
早泄是什么原因2. Gel purify digested plasmid using QIAquick Gel Extraction Kit and elute in EB. If BsmBI digested, a ~2kb filler piece should be prent on the gel. Only gel purify the larger band . Leave the 2kb band.
3. Phosphorylate and anneal each pair of oligos: 1 ul Oligo 1 (100 µM) 1 ul Oligo 2 (100 µM) 1 ul 10X T4 Ligation Buffer (NEB) 6.5 ul ddH 2O 0.5 ul T4 PNK (NEB M0201S) 10 ul total Plea u the T4 Ligation Buffer since the buffer supplied with the T4 PNK enzyme does not include ATP (or supplement to 1mM ATP).
会计专业求职信Put the phosphorylation/annealing reaction in a thermocycler using the following parameters: 37o C 30 min 95o C 5 min and then ramp down to 25o C at 5o C/min
4. Dilute annealed oligos from Step 3 at a 1:200 dilution into sterile water or EB.
5. Set up ligation reaction and incubate at room temperature for 10 min:潇洒风流
X ul BsmB I digested plasmid
from Step 2 (50ng)
1 ul diluted oligo duplex from Step 4 5 ul 2X Quick Liga Buffer (NEB) X ul ddH 2O 10 ul subtotal
1 ul Quick Liga (NEB M2200S) 11 ul total Also perform a negative control ligation (vector-only with water in place of oligos) and transformation. 6. Transformation into Stbl3 bacteria . Lentiviral transfer plasmids contain Long-Terminal Repeats (LTRs) and must be transformed into recombination-deficient bacteria. We u homemade Stbl3 (propagated from Invitrogen C7373-03) and get excellent plasmid yields. Although other RecA- strains may work, we have found the most consistent transformations and yields using Stbl3.中国古代婚礼