optimization screen preparation Search Results


droplet microfluidic screening  (ATCC)
95
ATCC droplet microfluidic screening
Droplet Microfluidic Screening, supplied by ATCC, used in various techniques. Bioz Stars score: 95/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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optimization screen preparation  (SPT Labtech)
95
SPT Labtech optimization screen preparation
Optimization Screen Preparation, supplied by SPT Labtech, used in various techniques. Bioz Stars score: 95/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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fda-approved drugs  (Chemdiv Inc)
90
Chemdiv Inc fda-approved drugs
Fda Approved Drugs, supplied by Chemdiv Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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tf20 microscope  (Thermo Fisher)
90
Thermo Fisher tf20 microscope
Tf20 Microscope, supplied by Thermo Fisher, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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tecan evo 100  (Tecan Systems)
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Tecan Systems tecan evo 100
Tecan Evo 100, supplied by Tecan Systems, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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human codon optimized cas9  (Addgene inc)
96
Addgene inc human codon optimized cas9
(A) Gene-specific sgRNA libraries were cloned into lentiviral plasmids containing barcoded <t>Cas9</t> effectors. After library transduction, K562 cells were sorted by target gene expression level into high- and low-expressing bins, and the relative frequency of sgRNA-Cas9 barcode pairs in both bins was compared. (B) Fold change of sgRNA representation in cell populations expressing high levels of the target gene compared with low-expressing cells, combined for all three genes tested. Only sgRNAs targeting CDS exons are shown. (C) Fold change of sgRNA representation grouped by 2 and 3 nt PAMs. Statistical significance was determined by comparing fold change of sgRNAs associated with a particular PAM with a respective non-targeting control using two-tailed Student’s t test with Bonferroni correction for multiple hypothesis testing. Error bars indicate standard error of the mean. Only statistically significant PAM/Cas9 combinations are shown in color. (D) CD46 ne9 gate, indicated with a dashed line, was set on the basis of K562 autofluorescence. Numbers displayed next to histograms indicate the percentage of cells in CD46 neg gate. LV, lentivirus. (E) Quantification of CD46 knockout in K562 cell line by lentiviral transduction of Cas9 nucleases and sgRNAs associated with NGG or NGH PAMs. Error bars indicate standard error of the mean.
Human Codon Optimized Cas9, supplied by Addgene inc, used in various techniques. Bioz Stars score: 96/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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mosquito robot  (SPT Labtech)
96
SPT Labtech mosquito robot
(A) Gene-specific sgRNA libraries were cloned into lentiviral plasmids containing barcoded <t>Cas9</t> effectors. After library transduction, K562 cells were sorted by target gene expression level into high- and low-expressing bins, and the relative frequency of sgRNA-Cas9 barcode pairs in both bins was compared. (B) Fold change of sgRNA representation in cell populations expressing high levels of the target gene compared with low-expressing cells, combined for all three genes tested. Only sgRNAs targeting CDS exons are shown. (C) Fold change of sgRNA representation grouped by 2 and 3 nt PAMs. Statistical significance was determined by comparing fold change of sgRNAs associated with a particular PAM with a respective non-targeting control using two-tailed Student’s t test with Bonferroni correction for multiple hypothesis testing. Error bars indicate standard error of the mean. Only statistically significant PAM/Cas9 combinations are shown in color. (D) CD46 ne9 gate, indicated with a dashed line, was set on the basis of K562 autofluorescence. Numbers displayed next to histograms indicate the percentage of cells in CD46 neg gate. LV, lentivirus. (E) Quantification of CD46 knockout in K562 cell line by lentiviral transduction of Cas9 nucleases and sgRNAs associated with NGG or NGH PAMs. Error bars indicate standard error of the mean.
Mosquito Robot, supplied by SPT Labtech, used in various techniques. Bioz Stars score: 96/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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ceta cmos detector  (Thermo Fisher)
90
Thermo Fisher ceta cmos detector
(A) Gene-specific sgRNA libraries were cloned into lentiviral plasmids containing barcoded <t>Cas9</t> effectors. After library transduction, K562 cells were sorted by target gene expression level into high- and low-expressing bins, and the relative frequency of sgRNA-Cas9 barcode pairs in both bins was compared. (B) Fold change of sgRNA representation in cell populations expressing high levels of the target gene compared with low-expressing cells, combined for all three genes tested. Only sgRNAs targeting CDS exons are shown. (C) Fold change of sgRNA representation grouped by 2 and 3 nt PAMs. Statistical significance was determined by comparing fold change of sgRNAs associated with a particular PAM with a respective non-targeting control using two-tailed Student’s t test with Bonferroni correction for multiple hypothesis testing. Error bars indicate standard error of the mean. Only statistically significant PAM/Cas9 combinations are shown in color. (D) CD46 ne9 gate, indicated with a dashed line, was set on the basis of K562 autofluorescence. Numbers displayed next to histograms indicate the percentage of cells in CD46 neg gate. LV, lentivirus. (E) Quantification of CD46 knockout in K562 cell line by lentiviral transduction of Cas9 nucleases and sgRNAs associated with NGG or NGH PAMs. Error bars indicate standard error of the mean.
Ceta Cmos Detector, supplied by Thermo Fisher, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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optimized antiretroviral drugs  (Tibotec Pharmaceuticals)
90
Tibotec Pharmaceuticals optimized antiretroviral drugs
(A) Gene-specific sgRNA libraries were cloned into lentiviral plasmids containing barcoded <t>Cas9</t> effectors. After library transduction, K562 cells were sorted by target gene expression level into high- and low-expressing bins, and the relative frequency of sgRNA-Cas9 barcode pairs in both bins was compared. (B) Fold change of sgRNA representation in cell populations expressing high levels of the target gene compared with low-expressing cells, combined for all three genes tested. Only sgRNAs targeting CDS exons are shown. (C) Fold change of sgRNA representation grouped by 2 and 3 nt PAMs. Statistical significance was determined by comparing fold change of sgRNAs associated with a particular PAM with a respective non-targeting control using two-tailed Student’s t test with Bonferroni correction for multiple hypothesis testing. Error bars indicate standard error of the mean. Only statistically significant PAM/Cas9 combinations are shown in color. (D) CD46 ne9 gate, indicated with a dashed line, was set on the basis of K562 autofluorescence. Numbers displayed next to histograms indicate the percentage of cells in CD46 neg gate. LV, lentivirus. (E) Quantification of CD46 knockout in K562 cell line by lentiviral transduction of Cas9 nucleases and sgRNAs associated with NGG or NGH PAMs. Error bars indicate standard error of the mean.
Optimized Antiretroviral Drugs, supplied by Tibotec Pharmaceuticals, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Image Search Results


(A) Gene-specific sgRNA libraries were cloned into lentiviral plasmids containing barcoded Cas9 effectors. After library transduction, K562 cells were sorted by target gene expression level into high- and low-expressing bins, and the relative frequency of sgRNA-Cas9 barcode pairs in both bins was compared. (B) Fold change of sgRNA representation in cell populations expressing high levels of the target gene compared with low-expressing cells, combined for all three genes tested. Only sgRNAs targeting CDS exons are shown. (C) Fold change of sgRNA representation grouped by 2 and 3 nt PAMs. Statistical significance was determined by comparing fold change of sgRNAs associated with a particular PAM with a respective non-targeting control using two-tailed Student’s t test with Bonferroni correction for multiple hypothesis testing. Error bars indicate standard error of the mean. Only statistically significant PAM/Cas9 combinations are shown in color. (D) CD46 ne9 gate, indicated with a dashed line, was set on the basis of K562 autofluorescence. Numbers displayed next to histograms indicate the percentage of cells in CD46 neg gate. LV, lentivirus. (E) Quantification of CD46 knockout in K562 cell line by lentiviral transduction of Cas9 nucleases and sgRNAs associated with NGG or NGH PAMs. Error bars indicate standard error of the mean.

Journal: Cell reports

Article Title: High-Throughput Screens of PAM-Flexible Cas9 Variants for Gene Knockout and Transcriptional Modulation

doi: 10.1016/j.celrep.2020.02.010

Figure Lengend Snippet: (A) Gene-specific sgRNA libraries were cloned into lentiviral plasmids containing barcoded Cas9 effectors. After library transduction, K562 cells were sorted by target gene expression level into high- and low-expressing bins, and the relative frequency of sgRNA-Cas9 barcode pairs in both bins was compared. (B) Fold change of sgRNA representation in cell populations expressing high levels of the target gene compared with low-expressing cells, combined for all three genes tested. Only sgRNAs targeting CDS exons are shown. (C) Fold change of sgRNA representation grouped by 2 and 3 nt PAMs. Statistical significance was determined by comparing fold change of sgRNAs associated with a particular PAM with a respective non-targeting control using two-tailed Student’s t test with Bonferroni correction for multiple hypothesis testing. Error bars indicate standard error of the mean. Only statistically significant PAM/Cas9 combinations are shown in color. (D) CD46 ne9 gate, indicated with a dashed line, was set on the basis of K562 autofluorescence. Numbers displayed next to histograms indicate the percentage of cells in CD46 neg gate. LV, lentivirus. (E) Quantification of CD46 knockout in K562 cell line by lentiviral transduction of Cas9 nucleases and sgRNAs associated with NGG or NGH PAMs. Error bars indicate standard error of the mean.

Article Snippet: In order to enable a meaningful comparison between different Cas9 variants, we used the human codon optimized Cas9 from lentiCRISPR v2 plasmid (Addgene 52961, ) as background forxCas9 and Cas9-NG mutations. xCas9 (also known asxCas3.7) mutations are as follows: A262T, R324L, S409I, E480K, E543D, M694I and E1219V ( ).

Techniques: Clone Assay, Transduction, Targeted Gene Expression, Expressing, Control, Two Tailed Test, Knock-Out

CD46 + A375 cells were transduced with lentivirus encoding the indicated Cas9 variants and sgRNAs targeting CD46 coding sequences. Target site PAMs are as indicated in each panel title. Following selection, CD46 negative cells were quantified by flow cytometry on the basis of the gate set on the unstained population at days 4, 7, 14, and 21. Standard error of the mean is shown (n = 3 replicate transductions).

Journal: Cell reports

Article Title: High-Throughput Screens of PAM-Flexible Cas9 Variants for Gene Knockout and Transcriptional Modulation

doi: 10.1016/j.celrep.2020.02.010

Figure Lengend Snippet: CD46 + A375 cells were transduced with lentivirus encoding the indicated Cas9 variants and sgRNAs targeting CD46 coding sequences. Target site PAMs are as indicated in each panel title. Following selection, CD46 negative cells were quantified by flow cytometry on the basis of the gate set on the unstained population at days 4, 7, 14, and 21. Standard error of the mean is shown (n = 3 replicate transductions).

Article Snippet: In order to enable a meaningful comparison between different Cas9 variants, we used the human codon optimized Cas9 from lentiCRISPR v2 plasmid (Addgene 52961, ) as background forxCas9 and Cas9-NG mutations. xCas9 (also known asxCas3.7) mutations are as follows: A262T, R324L, S409I, E480K, E543D, M694I and E1219V ( ).

Techniques: Transduction, Selection, Flow Cytometry

(A) Gating strategy for enumeration of K562 cells expressing the WT level of CD46 protein. No LV, no lentivirus. (B) Correlation between the frequency of alleles containing indels and the frequency of cells expressing the WT levels of CD46 protein. Dashed lines indicate 95% confidence intervals around the linear regression curve. NGG and NGH sgRNAs are included. r 2 is the Pearson coefficient of determination. (C) Relative frequency of deletions and insertions among edited alleles. Each line represents one sgRNA. Only NGG sgRNAs with >5% edited alleles are included. (D) Mean deletion and insertion sizes per Cas9 variant. Each data point represents the mean indel size for one sgRNA. Error bars indicate SEM. Only NGG sgRNAs with >5% edited reads are included. (E) Indel sizes (among edited reads) for each Cas9 variant.

Journal: Cell reports

Article Title: High-Throughput Screens of PAM-Flexible Cas9 Variants for Gene Knockout and Transcriptional Modulation

doi: 10.1016/j.celrep.2020.02.010

Figure Lengend Snippet: (A) Gating strategy for enumeration of K562 cells expressing the WT level of CD46 protein. No LV, no lentivirus. (B) Correlation between the frequency of alleles containing indels and the frequency of cells expressing the WT levels of CD46 protein. Dashed lines indicate 95% confidence intervals around the linear regression curve. NGG and NGH sgRNAs are included. r 2 is the Pearson coefficient of determination. (C) Relative frequency of deletions and insertions among edited alleles. Each line represents one sgRNA. Only NGG sgRNAs with >5% edited alleles are included. (D) Mean deletion and insertion sizes per Cas9 variant. Each data point represents the mean indel size for one sgRNA. Error bars indicate SEM. Only NGG sgRNAs with >5% edited reads are included. (E) Indel sizes (among edited reads) for each Cas9 variant.

Article Snippet: In order to enable a meaningful comparison between different Cas9 variants, we used the human codon optimized Cas9 from lentiCRISPR v2 plasmid (Addgene 52961, ) as background forxCas9 and Cas9-NG mutations. xCas9 (also known asxCas3.7) mutations are as follows: A262T, R324L, S409I, E480K, E543D, M694I and E1219V ( ).

Techniques: Expressing, Variant Assay

(A) Fold change of sgRNAs targeting the 3 kb region surrounding the primary TSS of CD45 gene. Only sgRNAs associated with an NGG PAM are displayed here (n = 123 sgRNAs). The regions with the strongest NGG sgRNA activity (indicated with dashed lines) were used to select sgRNAs (all PAMs) for subsequent analyses. CD45 transcript isoforms (PTPRC-204, PTPRC-215, PRPRC-201, PTPRC-209, PTPRC-206, and PTPRC-207) are shown in gray. (B) Fold-change of sgRNA representation grouped by 2 and 3 nt PAM categories. Statistical significance was determined by comparing fold change of sgRNAs associated with a particular PAM with a respective non-targeting control using two-sided Student’s t test with Bonferroni correction. Error bars indicate standard error of the mean. Only statistically significant PAM/Cas9 combinations are shown in color. CRISPRi: n = 2,165 sgRNAs; CRISPRa: n = 1,980 sgRNAs. (C) CD45 expression following CRISPR activation In the CD45 neg human A375 cell line. Only sgRNAs resulting In >1% CD45 pos cells with at least one Cas9 variant are displayed (see for data from all sgRNAs tested). Mean and individual values from three independent experiments are shown. For NAG and NAA PAMs, only one of three sgRNAs tested resulted in >1% CD45 pos cells. (D) Comparison of WT Cas9 and two PAM-flexible Cas9 variants across all three modalities tested in high-throughput screens. Fold-enrichment was calculated on the basis of the sgRNA frequency in the top bin over bottom bin; fold depletion was calculated on the basis of the sgRNA frequency in the bottom bin overtop bin. Only non-significant comparisons (ns, p > 0.05) are indicated; all other differences (between enzymes, within modalities) are significant.

Journal: Cell reports

Article Title: High-Throughput Screens of PAM-Flexible Cas9 Variants for Gene Knockout and Transcriptional Modulation

doi: 10.1016/j.celrep.2020.02.010

Figure Lengend Snippet: (A) Fold change of sgRNAs targeting the 3 kb region surrounding the primary TSS of CD45 gene. Only sgRNAs associated with an NGG PAM are displayed here (n = 123 sgRNAs). The regions with the strongest NGG sgRNA activity (indicated with dashed lines) were used to select sgRNAs (all PAMs) for subsequent analyses. CD45 transcript isoforms (PTPRC-204, PTPRC-215, PRPRC-201, PTPRC-209, PTPRC-206, and PTPRC-207) are shown in gray. (B) Fold-change of sgRNA representation grouped by 2 and 3 nt PAM categories. Statistical significance was determined by comparing fold change of sgRNAs associated with a particular PAM with a respective non-targeting control using two-sided Student’s t test with Bonferroni correction. Error bars indicate standard error of the mean. Only statistically significant PAM/Cas9 combinations are shown in color. CRISPRi: n = 2,165 sgRNAs; CRISPRa: n = 1,980 sgRNAs. (C) CD45 expression following CRISPR activation In the CD45 neg human A375 cell line. Only sgRNAs resulting In >1% CD45 pos cells with at least one Cas9 variant are displayed (see for data from all sgRNAs tested). Mean and individual values from three independent experiments are shown. For NAG and NAA PAMs, only one of three sgRNAs tested resulted in >1% CD45 pos cells. (D) Comparison of WT Cas9 and two PAM-flexible Cas9 variants across all three modalities tested in high-throughput screens. Fold-enrichment was calculated on the basis of the sgRNA frequency in the top bin over bottom bin; fold depletion was calculated on the basis of the sgRNA frequency in the bottom bin overtop bin. Only non-significant comparisons (ns, p > 0.05) are indicated; all other differences (between enzymes, within modalities) are significant.

Article Snippet: In order to enable a meaningful comparison between different Cas9 variants, we used the human codon optimized Cas9 from lentiCRISPR v2 plasmid (Addgene 52961, ) as background forxCas9 and Cas9-NG mutations. xCas9 (also known asxCas3.7) mutations are as follows: A262T, R324L, S409I, E480K, E543D, M694I and E1219V ( ).

Techniques: Activity Assay, Control, Expressing, CRISPR, Activation Assay, Variant Assay, Comparison, High Throughput Screening Assay

(A) Crystal structures of Cas9 mutants. xCas9 mutations are shown on a WT Cas9 structure (PDB: 4un3; ). xCas9-NG mutations are displayed on a Cas9-NG structure (PDB: 6ai6; ). The sgRNA is shown in black, and the target DNA is shown in blue. (B and C) Knockout (B) and activation (C) activity for individual sgRNAs with target sites with the indicated PAMs. Each xCas9 or xCas9-NG experiment was normalized to Cas9-NG on a per-sgRNA basis. Only sgRNAs resulting in >1% knockout or activation are shown. Non-normalized data for xCas9 and Cas9-NG are displayed in and and are included here for comparison with xCas9-NG. ns, p > 0.05; *p < 0.05, **p < 0.01, and ****p < 0.0001

Journal: Cell reports

Article Title: High-Throughput Screens of PAM-Flexible Cas9 Variants for Gene Knockout and Transcriptional Modulation

doi: 10.1016/j.celrep.2020.02.010

Figure Lengend Snippet: (A) Crystal structures of Cas9 mutants. xCas9 mutations are shown on a WT Cas9 structure (PDB: 4un3; ). xCas9-NG mutations are displayed on a Cas9-NG structure (PDB: 6ai6; ). The sgRNA is shown in black, and the target DNA is shown in blue. (B and C) Knockout (B) and activation (C) activity for individual sgRNAs with target sites with the indicated PAMs. Each xCas9 or xCas9-NG experiment was normalized to Cas9-NG on a per-sgRNA basis. Only sgRNAs resulting in >1% knockout or activation are shown. Non-normalized data for xCas9 and Cas9-NG are displayed in and and are included here for comparison with xCas9-NG. ns, p > 0.05; *p < 0.05, **p < 0.01, and ****p < 0.0001

Article Snippet: In order to enable a meaningful comparison between different Cas9 variants, we used the human codon optimized Cas9 from lentiCRISPR v2 plasmid (Addgene 52961, ) as background forxCas9 and Cas9-NG mutations. xCas9 (also known asxCas3.7) mutations are as follows: A262T, R324L, S409I, E480K, E543D, M694I and E1219V ( ).

Techniques: Knock-Out, Activation Assay, Activity Assay, Comparison

KEY RESOURCES TABLE

Journal: Cell reports

Article Title: High-Throughput Screens of PAM-Flexible Cas9 Variants for Gene Knockout and Transcriptional Modulation

doi: 10.1016/j.celrep.2020.02.010

Figure Lengend Snippet: KEY RESOURCES TABLE

Article Snippet: In order to enable a meaningful comparison between different Cas9 variants, we used the human codon optimized Cas9 from lentiCRISPR v2 plasmid (Addgene 52961, ) as background forxCas9 and Cas9-NG mutations. xCas9 (also known asxCas3.7) mutations are as follows: A262T, R324L, S409I, E480K, E543D, M694I and E1219V ( ).

Techniques: Virus, Recombinant, DNA Extraction, DNA Purification, Staining, Plasmid Preparation, Software