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Published byShannon Ellis Modified over 9 years ago
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Last class Overall goal for labs 7-9 How to pick candidate miRNA targets Overview: “Validate” target prediction
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Lab 8 Hard copy: Plasmid worksheets!
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Labs 7-9 flow chart Pick target Design primers Isolate RNA from cells Make cDNA using RT-PCR Use qPCR to quantify expression level Repeat
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RNA Isolation: Overview ? ? ? http://www.thermoscientificbio.com/uploadedImages/Products/Nucleic_Acid_Purification/Kits_-_Genomics/D_RNA_cleanup_and_concentration_protocol.jpg
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The RT reaction What are components for RT reaction?
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Controls RTPCR RT PCR RT PCR
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Controls -RTPCR -RT PCR -RT PCR
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Lab session Each group will start with either miRNA or Control Make total RNA (freeze half!) Remaining: Split into TWO tubes Keep one, swap one with another group Make cDNA
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Lab session Group A Control Control RNA Group B miRNA miRNA RNA Control RNAmiRNA RNAControl RNAmiRNA RNA
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Quantifying DNA/RNA: qPCR 1 cycle 2 cycles 3 cycles 30 cycles Start with 1 moleculeStart with 10 molecules
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Same starting material… http://www.sabiosciences.com
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Different starting material… http://www.sabiosciences.com
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Solution: qPCR http://www.abbottmolecular.com
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“Threshold” cycle http://www.sabiosciences.com
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“Threshold” cycle http://www.sabiosciences.com
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How can we quantify DNA in PCR? DNA molecules in PCR How to quantify ONLY product?
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TemplatePrimerdNTPs Quantifying PCR products TemplatePrimerdNTPsProduct
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qPCR controls Normalize amount of starting material? Could normalize total RNA Better method?
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qPCR controls Normalize for overexpression of miR-23b? Positive control
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“Threshold” cycle http://www.sabiosciences.com
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Calculations C T = C T (control) - C T (miR) C T (miR) = C T (target-miR) - C T (endogenous control-miR) C T (control) = C T (target-control) - C T (endogenous control-control) Expression fold change = 2 C T
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Other roles of RNAs What can you use complementarity for?
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