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Anti epcam1 clone g8

Manufactured by Thermo Fisher Scientific
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The Anti-EpCAM1 clone G8.8 is a laboratory reagent used for the detection and analysis of the EpCAM1 protein. It is designed for research use only and its core function is to bind to the EpCAM1 molecule, enabling its identification and quantification in various biological samples.

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Lab products found in correlation

Anti cd80 clone 16 10a1, by BioLegend (3 mentions) Streptavidin pe cy7, by Thermo Fisher Scientific (3 mentions) Anti cd45 clone 30 f11, by Thermo Fisher Scientific (3 mentions) Anti ly51 clone 6c3, by BioLegend (3 mentions) Cd104 clone 346 11a, by BioLegend (3 mentions) Facsaria fusion 1 cell sorter, by BD (3 mentions) Biotinylated uea 1, by Vector Laboratories (3 mentions) Anti mhc 2 clone m5 114, by Thermo Fisher Scientific (3 mentions) Lsrfortessa, by BD (3 mentions) Dnase 1, by Roche (3 mentions) Collagenase dispase, by Roche (3 mentions) Anti cd45 beads, by Miltenyi Biotec (2 mentions) Ls column, by Miltenyi Biotec (2 mentions)

Close spelling variants of this product

Clone G8.8

3 protocols using anti epcam1 clone g8

1

Thymic Epithelial Cell Isolation and Analysis

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For thymic epithelial cell analysis, single cell suspensions were generated by digesting thymic lobes with collagenase dispase (2.5mg/ml, Roche) and DNase 1 (40mg/ml Roche). CD45- cells were enriched by the depletion of CD45+ cells using anti-CD45 beads and LS columns (Miltenyi Biotec). The following antibodies were used for TEC analysis: anti-CD45 clone 30-F11 (eBioscience), anti-EpCAM1 clone G8.8 (eBioscience), anti-Ly51 clone 6C3 (Biolegend), anti-MHCII clone M5/114.15.2 (eBioscience), anti-CD80 clone 16-10A1 (Biolegend), CD104 clone 346-11A (Biolegend), and anti-MHCI 28-14-8. Biotinylated UEA-1 (Vector laboratories) was detected using streptavidin PECy7 (eBioscience). Cells were analysed using a LSR Fortessa (Becton Dickinson) with data analysis carried out using Flowjo v10 (Becton Dickinson). For cell sorting, TEC subsets were identified using the antibodies above, and isolated using a FACS Aria Fusion 1 cell sorter (Becton Dickinson).
The sorting strategy for the different TEC subsets were as follows, Cxcl12DsRed+ cTEC: CD45-EpCAM1+UEA1-Ly51+CXCL12DsRed+; CXCL12DsRed- cTEC: CD45-EpCAM1+UEA1-Ly51+CXCL12DsRed-; mTEClo: CD45-EpCAM1+UEA1+Ly51-CD80-MHCII-; mTEChi: CD45-EpCAM1+UEA-1-Ly51+CD80+MHCII+; CD104+ mTEClo, CD45-EpCAM1+UEA1+Ly51-CD80-MHCII-CD104+; CD104- mTEClo, CD45-EpCAM1+UEA1+Ly51-CD80-MHCII-CD104-.
White A.J., Parnell S.M., Handel A., Maio S., Bacon A., Cosway E.J., Lucas B., James K.D., Cowan J.E., Jenkinson W.E., Hollander G.A, & Anderson G. (2023). Diversity in Cortical Thymic Epithelial Cells Occurs through Loss of a Foxn1-Dependent Gene Signature Driven by Stage-Specific Thymocyte Cross-Talk. The Journal of Immunology Author Choice, 210(1), 40-49.
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2

Isolation and Flow Cytometry Analysis of Thymic Epithelial Cells

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For TEC analysis, single-cell suspensions were generated by digesting thymic lobes with collagenase Dispase (2.5 mg/ml; Roche) and DNase 1 (40 mg/ml; Roche). CD45 cells were enriched by the depletion of CD45+ cells using anti-CD45 beads and LS columns (Miltenyi Biotec). The following Abs were used for TEC analysis: anti-CD45 clone 30-F11 (eBioscience), anti-EpCAM1 clone G8.8 (eBioscience), anti-Ly51 clone 6C3 (BioLegend), anti–MHC II clone M5/114.15.2 (eBioscience), anti-CD80 clone 16-10A1 (BioLegend), CD104 clone 346-11A (BioLegend), and anti–MHC I 28-14-8. Biotinylated UEA-1 (Vector laboratories) was detected using streptavidin PECy7 (eBioscience). Cells were analyzed using a LSR Fortessa (Becton Dickinson) with data analysis carried out using FlowJo v10 (Becton Dickinson). For cell sorting, TEC subsets were identified using the earlier Abs and isolated using a FACSAria Fusion 1 cell sorter (Becton Dickinson). The sorting strategy for the different TEC subsets was as follows: Cxcl12DsRed+ cTEC, CD45EpCAM1+UEA1Ly51+CXCL12DsRed+; CXCL12DsRed− cTEC, CD45EpCAM1+UEA1Ly51+CXCL12DsRed−; mTEClo, CD45EpCAM1+UEA1+Ly51CD80MHC II; mTEChi, CD45EpCAM1+UEA+Ly51CD80+MHC II+; CD104+ mTEClo, CD45EpCAM1+UEA1+Ly51CD80MHC IICD104+; and CD104 mTEClo, CD45EpCAM1+UEA1+Ly51CD80MHC IICD104.
White A.J., Parnell S.M., Handel A., Maio S., Bacon A., Cosway E.J., Lucas B., James K.D., Cowan J.E., Jenkinson W.E., Hollander G.A, & Anderson G. (2023). Diversity in Cortical Thymic Epithelial Cells Occurs through Loss of a Foxn1-Dependent Gene Signature Driven by Stage-Specific Thymocyte Cross-Talk. The Journal of Immunology Author Choice, 210(1), 40-49.
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3

Isolation and Flow Cytometry Analysis of Thymic Epithelial Cells

Check if the same lab product or an alternative is used in the 5 most similar protocols
For TEC analysis, single-cell suspensions were generated by digesting thymic lobes with collagenase Dispase (2.5 mg/ml; Roche) and DNase 1 (40 mg/ml; Roche). CD45 cells were enriched by the depletion of CD45+ cells using anti-CD45 beads and LS columns (Miltenyi Biotec). The following Abs were used for TEC analysis: anti-CD45 clone 30-F11 (eBioscience), anti-EpCAM1 clone G8.8 (eBioscience), anti-Ly51 clone 6C3 (BioLegend), anti–MHC II clone M5/114.15.2 (eBioscience), anti-CD80 clone 16-10A1 (BioLegend), CD104 clone 346-11A (BioLegend), and anti–MHC I 28-14-8. Biotinylated UEA-1 (Vector laboratories) was detected using streptavidin PECy7 (eBioscience). Cells were analyzed using a LSR Fortessa (Becton Dickinson) with data analysis carried out using FlowJo v10 (Becton Dickinson). For cell sorting, TEC subsets were identified using the earlier Abs and isolated using a FACSAria Fusion 1 cell sorter (Becton Dickinson). The sorting strategy for the different TEC subsets was as follows: Cxcl12DsRed+ cTEC, CD45EpCAM1+UEA1Ly51+CXCL12DsRed+; CXCL12DsRed− cTEC, CD45EpCAM1+UEA1Ly51+CXCL12DsRed−; mTEClo, CD45EpCAM1+UEA1+Ly51CD80MHC II; mTEChi, CD45EpCAM1+UEA+Ly51CD80+MHC II+; CD104+ mTEClo, CD45EpCAM1+UEA1+Ly51CD80MHC IICD104+; and CD104 mTEClo, CD45EpCAM1+UEA1+Ly51CD80MHC IICD104.
White A.J., Parnell S.M., Handel A., Maio S., Bacon A., Cosway E.J., Lucas B., James K.D., Cowan J.E., Jenkinson W.E., Hollander G.A, & Anderson G. (2023). Diversity in Cortical Thymic Epithelial Cells Occurs through Loss of a Foxn1-Dependent Gene Signature Driven by Stage-Specific Thymocyte Cross-Talk. The Journal of Immunology Author Choice, 210(1), 40-49.
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