Please answer Discuss if you could perform the PCR and then agarose gel electrophoresis using a coding gene instead of a VNTR
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- what is the |usage of DNA separation in gel electrophoresis please write the resources under the answeracconline.austincc.edu/ultra/courses/_891351_1/cl/outline O gel electrophoresis O PCR O genomic library DNA microarray A patient is suspected of having a certain type of cancer that involves several genes. Doctors want to determine whether this patient is expressing these cancer genes and to what leve each gene is being expressed. What technique may be used? O molecular cloning O CRISPR gene editing 5 genetic recombination that occurs naturally (think horizontal gene transfer, meioșis, fertilization, or mutations). Ar : Y EV АУ ΩΘΙ 用く X A MacBook Air & 8 88 Q V Ix % 0 8A EXE D B 图 Q 用图 5 d Show All † 19 EHR Immunizavalidate Mega CRISPR with CRISPR
- What type of probe is used for real-time PCR? Explain howthe level of fluorescence correlates with the amount of PCRproduct.You need to complete the following steps for an experiment. Explain whether an acrylamide gel or an agarose gel is more appropriate to use for the following experiments. Purifying tRNA from total RNA Isolating a vector insert for cloning Analyzing PCR productsWhat type of probe is used for real-time PCR? Explain howthe level of fluorescence correlates with the level of PCRproduct.
- Why uncut and cut PCR at different position in the agarose gel? which one can be decided accuracy the size of PCR?Please submit a paragraph comparing two methods of DNA isolation (traditional with Qaigen DNA isolation kit method).Make the PCR Cocktail This table lists the ingredients, stock reagent concentrations, and concentrations in the PCR reaction. Prepare a "PCR cocktail" to be added to your samples to achieve these concentrations. Make enough cocktail to run nine samples. [Four student samples + three positive controls + one negative control + one extra.] {Hint: Remember that the concentration in the reaction is not the same as the concentration in the cocktail!] Component Stock Concentration Concentration in the PCR reaction Volume per reaction Volume to make cocktail Sterile water - - µl µl PCR buffer w/ MgCl2 10x 1x µl µl Nucleotide mix 10 mM 0.2 mM µl µl Primer 1 (Forward) 10 µM 1.0 µM µl µl Primer 2 (Reverse) 10 µM 1.0 µM µl µl Taq DNA polymerase 5 U/µl 1.0 U µl µl DNA template (sample) - ~1 ng 20 µl µl Total - - 40 µl µl
- Answer the following questions related to PCR Bioinformatics for DNA Extraction using Why is it necessary to chelate the metal ions from the solution during the boiling/lysis step at 100 degrees celsius? What would happen if you did not use a chelating agent such as the InstaGene matrix? What is needed from the cells for PCR? What structures must be broken to release the DNA from a cell?This is what the LAB FLOW would look like: CULTURE BACTERIA EXTRACT RNA RANDOM HEXAMER REVERSE TRANSCRIPTION OF RNA PCR OF lacZ GENE ELECTROPHORESIS If you wanted to prepare only one PCR reaction, how much of each reagent would you add to the PCR tube? What would be the final primer concentration if 0.5 μl of 10 μM primers were added to a PCR reaction with a final volume of 20 μl?Select all that would be true if I had a missense mutation in an gene: The missense mutant protein would be the same size by Western as the wildtype protein The missense mutant allele would be a different size compared to wildtype by PCR- electrophoresis The missense mutant protein would be a different size by Western compared to the wildtype protein The missense mutant allele would be the same size as wildtype by PCR-electrophoresis