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Genechip mouse gene st 1.0 array chip

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The GeneChip Mouse Gene ST 1.0 Array is a gene expression microarray designed for the analysis of the mouse transcriptome. The array contains probes targeting mouse gene transcripts, allowing for the measurement of gene expression levels across the mouse genome.

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Lab products found in correlation

Wt ovation pico rna amplification system, by Tecan (2 mentions) Genespring gx11, by Agilent Technologies (2 mentions) Trizol rna isolation, by Thermo Fisher Scientific (2 mentions) Rneasy mini kit, by Qiagen (2 mentions) Agilent 2100 bioanalyzer, by Agilent Technologies (2 mentions) Facsaria, by BD (2 mentions)

4 protocols using genechip mouse gene st 1.0 array chip

1

Microarray Analysis of Intestinal Eosinophils

Cited 2 times
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Microarray analysis on sorted intestinal eosinophils was performed as previously described.56 (link) Small intestinal eosinophils were sorted as DAPICCR3+SiglecF+CD45+CD4CD8aCD19B220SSChigh cells from 10 animals using FACS Aria (BD). Total RNA from sorted eosinophils was extracted by standard TRIzol RNA isolation (Invitrogen) and subsequently column-purified with an RNeasy Mini Kit (Qiagen). mRNA integrity was validated by the Agilent 2100 bio-analyzer (Agilent Technologies). Eosinophil mRNA was amplified and labeled with the WT-Ovation Pico RNA Amplification System (NuGen) and subjected to the GeneChip Mouse Gene ST 1.0 Array chip (Affymetrix). Microarray expression analysis was performed at Cincinnati Children’s Hospital Medical Center’s Chip Core facility, and expression data were analyzed by the software of Genespring GX 11 (Agilent Technologies). The Affymetrix raw expression values were filtered with the significance threshold of 400 as previously reported56 (link),57 (link) and validated by the levels of eosinophil-specific major basic protein gene (also known as proteoglycan 2 [Prg2]) and eosinophil non-expressed glucagon (Gcg) (Fig. S12).
Jung Y., Wen T., Mingler M., Caldwell J., Wang Y., Chaplin D., Lee E., Jang M., Woo S., Seoh J., Miyasaka M, & Rothenberg M. (2015). IL-1β in eosinophil-mediated small intestinal homeostasis and IgA production. Mucosal immunology, 8(4), 930-942.
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2

Microarray Analysis of Intestinal Eosinophils

Cited 2 times
Check if the same lab product or an alternative is used in the 5 most similar protocols
Microarray analysis on sorted intestinal eosinophils was performed as previously described.56 (link) Small intestinal eosinophils were sorted as DAPICCR3+SiglecF+CD45+CD4CD8aCD19B220SSChigh cells from 10 animals using FACS Aria (BD). Total RNA from sorted eosinophils was extracted by standard TRIzol RNA isolation (Invitrogen) and subsequently column-purified with an RNeasy Mini Kit (Qiagen). mRNA integrity was validated by the Agilent 2100 bio-analyzer (Agilent Technologies). Eosinophil mRNA was amplified and labeled with the WT-Ovation Pico RNA Amplification System (NuGen) and subjected to the GeneChip Mouse Gene ST 1.0 Array chip (Affymetrix). Microarray expression analysis was performed at Cincinnati Children’s Hospital Medical Center’s Chip Core facility, and expression data were analyzed by the software of Genespring GX 11 (Agilent Technologies). The Affymetrix raw expression values were filtered with the significance threshold of 400 as previously reported56 (link),57 (link) and validated by the levels of eosinophil-specific major basic protein gene (also known as proteoglycan 2 [Prg2]) and eosinophil non-expressed glucagon (Gcg) (Fig. S12).
Jung Y., Wen T., Mingler M., Caldwell J., Wang Y., Chaplin D., Lee E., Jang M., Woo S., Seoh J., Miyasaka M, & Rothenberg M. (2015). IL-1β in eosinophil-mediated small intestinal homeostasis and IgA production. Mucosal immunology, 8(4), 930-942.
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3

Pax4 Transgenic Islet Gene Expression

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Labelled cRNA samples were prepared from pools of at least 100 islets isolated from either Pax4/rtTA or Pax4R121W/rtTA transgenic animals (8-week-old females) treated with DOX or not treated [14 (link)]. Three preparations of cRNA per group were then hybridised to the GeneChip Mouse Gene 1.0 ST Array chip (Affymetrix, Santa Clara, CA, USA) using the standard protocols of the Genomic Core Facility, CABIMER. Raw data are accessible in the Gene Expression Omnibus database under accession number GSE62846, while its analysis is described in ESM Methods.
Mellado-Gil J.M., Jiménez-Moreno C.M., Martin-Montalvo A., Alvarez-Mercado A.I., Fuente-Martin E., Cobo-Vuilleumier N., Lorenzo P.I., Bru-Tari E., de Gracia Herrera-Gómez I., López-Noriega L., Pérez-Florido J., Santoyo-López J., Spyrantis A., Meda P., Boehm B.O., Quesada I, & Gauthier B.R. (2016). PAX4 preserves endoplasmic reticulum integrity preventing beta cell degeneration in a mouse model of type 1 diabetes mellitus. Diabetologia, 59, 755-765.
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4

Transcriptional Profiling of Pax4/rtTA Islets

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Labeled cRNA samples were prepared from pools of at least 100 islets isolated from Pax4/rtTA transgenic animals (8-week old females) treated or not with DOX as previously described17 (link). Three independent preparations of cRNA per group were then hybridized to the GeneChip Mouse Gene 1.0 ST Array chip (Affymetrix, Santa Clara, CA) using standard protocols of the Genomic Core Facility of CABIMER. Analysis of the transcriptome profiling is described elsewhere (Mellado Gil et al., Manuscript submitted). Raw data are accessible in the Gene Expression Omnibus database under accession number GSE62846.
Lorenzo P.I., Fuente-Martín E., Brun T., Cobo-Vuilleumier N., Jimenez-Moreno C.M., G. Herrera Gomez I., López Noriega L., Mellado-Gil J.M., Martin-Montalvo A., Soria B, & Gauthier B.R. (2015). PAX4 Defines an Expandable β-Cell Subpopulation in the Adult Pancreatic Islet. Scientific Reports, 5, 15672.
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