multiplex primer extension assay Search Results


multiplex primer extension assay  (Sequenom)
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Sequenom multiplex primer extension assay
Multiplex Primer Extension Assay, supplied by Sequenom, 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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multiplex primer extension/denaturing hplc assay  (Transgenomic)
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Transgenomic multiplex primer extension/denaturing hplc assay
Multiplex Primer Extension/Denaturing Hplc Assay, supplied by Transgenomic, 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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primer extension of multiplex products  (Sequenom)
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Sequenom primer extension of multiplex products
Primer Extension Of Multiplex Products, supplied by Sequenom, 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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multiplex extension primers ( )  (agena bioscience)
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multiplexed primer extension (iplex)  (agena bioscience)
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agena bioscience multiplexed primer extension (iplex)
Multiplexed Primer Extension (Iplex), supplied by agena bioscience, 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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multiplexed primer extension method  (Sequenom)
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Sequenom multiplexed primer extension method
Multiplexed Primer Extension Method, supplied by Sequenom, 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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mass array system to design multiplex reactions for pcr and iplex primer extension  (Sequenom)
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Sequenom mass array system to design multiplex reactions for pcr and iplex primer extension
Mass Array System To Design Multiplex Reactions For Pcr And Iplex Primer Extension, supplied by Sequenom, 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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multiplex rna-single nucleotide primer extension (snupe) assays  (Sequenom)
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Sequenom multiplex rna-single nucleotide primer extension (snupe) assays
Testing for transgenerational epigenetic inheritance of the aberrant imprinted expression. (A) Breeding design to test whether ED-perturbed parental allele-specific transcription is transgenerationally inherited through the paternal germline to an unexposed generation. G1 male fetuses were exposed in utero to EDs or vehicle control (‘oil’) daily from 12.5 dpc to 16.5 dpc. After reaching adulthood, 129S1 G1 males were mated with 129S1 unexposed females to generate G2 offspring (3 blue stars), which derived from exposed prospermatogonia. At adulthood, G2 males were mated with unexposed JF1 females to generate G3 offspring, which were never directly exposed to EDs. JF1 × 129 G3 fetuses were dissected at 13.5 dpc to collect organs for <t>RNA</t> isolation. Parental-specific transcription was quantified in the total RNA using multiplex <t>SNuPE</t> assays. (B) Results of Sequenom allelotyping experiments using heart and lung tissue of the G3 generation; color scale as in Figure ; letters in parentheses denote independent SNPs. Notice the lack of inherited changes from the exposed generation. More groups of fetuses are shown in Additional file . This Figure includes standards that are routinely included in the Sequenom runs (see Methods).
Multiplex Rna Single Nucleotide Primer Extension (Snupe) Assays, supplied by Sequenom, 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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sequencing primers for the multiplex single-base extension (sbe) reaction  (Qiagen)
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Qiagen sequencing primers for the multiplex single-base extension (sbe) reaction
Testing for transgenerational epigenetic inheritance of the aberrant imprinted expression. (A) Breeding design to test whether ED-perturbed parental allele-specific transcription is transgenerationally inherited through the paternal germline to an unexposed generation. G1 male fetuses were exposed in utero to EDs or vehicle control (‘oil’) daily from 12.5 dpc to 16.5 dpc. After reaching adulthood, 129S1 G1 males were mated with 129S1 unexposed females to generate G2 offspring (3 blue stars), which derived from exposed prospermatogonia. At adulthood, G2 males were mated with unexposed JF1 females to generate G3 offspring, which were never directly exposed to EDs. JF1 × 129 G3 fetuses were dissected at 13.5 dpc to collect organs for <t>RNA</t> isolation. Parental-specific transcription was quantified in the total RNA using multiplex <t>SNuPE</t> assays. (B) Results of Sequenom allelotyping experiments using heart and lung tissue of the G3 generation; color scale as in Figure ; letters in parentheses denote independent SNPs. Notice the lack of inherited changes from the exposed generation. More groups of fetuses are shown in Additional file . This Figure includes standards that are routinely included in the Sequenom runs (see Methods).
Sequencing Primers For The Multiplex Single Base Extension (Sbe) Reaction, supplied by Qiagen, 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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multiplex primer extension-based method  (Pharmatech)
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Pharmatech multiplex primer extension-based method
Testing for transgenerational epigenetic inheritance of the aberrant imprinted expression. (A) Breeding design to test whether ED-perturbed parental allele-specific transcription is transgenerationally inherited through the paternal germline to an unexposed generation. G1 male fetuses were exposed in utero to EDs or vehicle control (‘oil’) daily from 12.5 dpc to 16.5 dpc. After reaching adulthood, 129S1 G1 males were mated with 129S1 unexposed females to generate G2 offspring (3 blue stars), which derived from exposed prospermatogonia. At adulthood, G2 males were mated with unexposed JF1 females to generate G3 offspring, which were never directly exposed to EDs. JF1 × 129 G3 fetuses were dissected at 13.5 dpc to collect organs for <t>RNA</t> isolation. Parental-specific transcription was quantified in the total RNA using multiplex <t>SNuPE</t> assays. (B) Results of Sequenom allelotyping experiments using heart and lung tissue of the G3 generation; color scale as in Figure ; letters in parentheses denote independent SNPs. Notice the lack of inherited changes from the exposed generation. More groups of fetuses are shown in Additional file . This Figure includes standards that are routinely included in the Sequenom runs (see Methods).
Multiplex Primer Extension Based Method, supplied by Pharmatech, 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


Testing for transgenerational epigenetic inheritance of the aberrant imprinted expression. (A) Breeding design to test whether ED-perturbed parental allele-specific transcription is transgenerationally inherited through the paternal germline to an unexposed generation. G1 male fetuses were exposed in utero to EDs or vehicle control (‘oil’) daily from 12.5 dpc to 16.5 dpc. After reaching adulthood, 129S1 G1 males were mated with 129S1 unexposed females to generate G2 offspring (3 blue stars), which derived from exposed prospermatogonia. At adulthood, G2 males were mated with unexposed JF1 females to generate G3 offspring, which were never directly exposed to EDs. JF1 × 129 G3 fetuses were dissected at 13.5 dpc to collect organs for RNA isolation. Parental-specific transcription was quantified in the total RNA using multiplex SNuPE assays. (B) Results of Sequenom allelotyping experiments using heart and lung tissue of the G3 generation; color scale as in Figure ; letters in parentheses denote independent SNPs. Notice the lack of inherited changes from the exposed generation. More groups of fetuses are shown in Additional file . This Figure includes standards that are routinely included in the Sequenom runs (see Methods).

Journal: Genome Biology

Article Title: Deleterious effects of endocrine disruptors are corrected in the mammalian germline by epigenome reprogramming

doi: 10.1186/s13059-015-0619-z

Figure Lengend Snippet: Testing for transgenerational epigenetic inheritance of the aberrant imprinted expression. (A) Breeding design to test whether ED-perturbed parental allele-specific transcription is transgenerationally inherited through the paternal germline to an unexposed generation. G1 male fetuses were exposed in utero to EDs or vehicle control (‘oil’) daily from 12.5 dpc to 16.5 dpc. After reaching adulthood, 129S1 G1 males were mated with 129S1 unexposed females to generate G2 offspring (3 blue stars), which derived from exposed prospermatogonia. At adulthood, G2 males were mated with unexposed JF1 females to generate G3 offspring, which were never directly exposed to EDs. JF1 × 129 G3 fetuses were dissected at 13.5 dpc to collect organs for RNA isolation. Parental-specific transcription was quantified in the total RNA using multiplex SNuPE assays. (B) Results of Sequenom allelotyping experiments using heart and lung tissue of the G3 generation; color scale as in Figure ; letters in parentheses denote independent SNPs. Notice the lack of inherited changes from the exposed generation. More groups of fetuses are shown in Additional file . This Figure includes standards that are routinely included in the Sequenom runs (see Methods).

Article Snippet: This allowed measurement of the allele-specific transcription of known imprinted genes in JF1 × OG2 cells using multiplex RNA-single nucleotide primer extension (SNuPE) assays uisng Sequenom allelotyping [ ].

Techniques: Expressing, In Utero, Derivative Assay, Isolation, Multiplex Assay