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Image Search Results
Journal: Current protocols in human genetics
Article Title: In vivo and In vitro methods to identify DNA sequence variants that alter RNA Splicing
doi: 10.1002/cphg.60
Figure Lengend Snippet: In PCR #1, a 500 bp test sequence and 225 bp SV40PA sequence are added to the same reaction to form a test sequence-SV40PA combined construct. In PCR #2, the PCR #1 product and a 600 bp CMV Promoter are added to the same reaction to form the full minigene construct. Overlapping, homologous regions of these gene fragments allow for assembly to occur.
Article Snippet: Tris EDTA Suspension Buffer (10 mM Tris, 0.1 mM EDTA, pH 8.0) Nuclease-Free H20 (ThermoFisher Scientific Cat. No. AM9932) Primers for PCR #1 reaction: N500-RTPCR-F2,
Techniques: Sequencing, Construct
Journal: Current protocols in human genetics
Article Title: In vivo and In vitro methods to identify DNA sequence variants that alter RNA Splicing
doi: 10.1002/cphg.60
Figure Lengend Snippet: gBlocks and other primers used in laboratory protocols
Article Snippet: Tris EDTA Suspension Buffer (10 mM Tris, 0.1 mM EDTA, pH 8.0) Nuclease-Free H20 (ThermoFisher Scientific Cat. No. AM9932) Primers for PCR #1 reaction: N500-RTPCR-F2,
Techniques: Sequencing, Multiplexing, Amplification
Journal: Current protocols in human genetics
Article Title: In vivo and In vitro methods to identify DNA sequence variants that alter RNA Splicing
doi: 10.1002/cphg.60
Figure Lengend Snippet: PCR #1 set up. Repeat for as many gBlocks as are required.
Article Snippet: Tris EDTA Suspension Buffer (10 mM Tris, 0.1 mM EDTA, pH 8.0) Nuclease-Free H20 (ThermoFisher Scientific Cat. No. AM9932) Primers for PCR #1 reaction: N500-RTPCR-F2,
Techniques: Concentration Assay, Sequencing, Construct
Journal: Current protocols in human genetics
Article Title: In vivo and In vitro methods to identify DNA sequence variants that alter RNA Splicing
doi: 10.1002/cphg.60
Figure Lengend Snippet: 15 lanes containing independent PCR #1 products are shown. Each band is approximately 650-700 bp in size, and represents an individual test sequence (500 bp) attached to a SV40PA signal (225 bp). Note that products seem to be migrating to the same positions in pairs, as would be expected with reference and alternate containing test sequences that have identical lengths.
Article Snippet: Tris EDTA Suspension Buffer (10 mM Tris, 0.1 mM EDTA, pH 8.0) Nuclease-Free H20 (ThermoFisher Scientific Cat. No. AM9932) Primers for PCR #1 reaction: N500-RTPCR-F2,
Techniques: Sequencing
Journal: Current protocols in human genetics
Article Title: In vivo and In vitro methods to identify DNA sequence variants that alter RNA Splicing
doi: 10.1002/cphg.60
Figure Lengend Snippet: PCR #2 set up. Repeat for as many gBlocks as are required.
Article Snippet: Tris EDTA Suspension Buffer (10 mM Tris, 0.1 mM EDTA, pH 8.0) Nuclease-Free H20 (ThermoFisher Scientific Cat. No. AM9932) Primers for PCR #1 reaction: N500-RTPCR-F2,
Techniques: Concentration Assay
Journal: Current protocols in human genetics
Article Title: In vivo and In vitro methods to identify DNA sequence variants that alter RNA Splicing
doi: 10.1002/cphg.60
Figure Lengend Snippet: Amplification of CMVp-N500
Article Snippet: Tris EDTA Suspension Buffer (10 mM Tris, 0.1 mM EDTA, pH 8.0) Nuclease-Free H20 (ThermoFisher Scientific Cat. No. AM9932) Primers for PCR #1 reaction: N500-RTPCR-F2,
Techniques: Amplification, Concentration Assay, Sequencing