Recall that you used agarose powder, 1X TBE buffer, and a fluorescent dye, GreenGlo, to make...

When adding your DNA samples to the agarose gel, you will need to add loading dye...

When adding your DNA samples to the agarose gel, you will need to add loading dye to the samples. Loading dye contains: ¥ glycerol, which helps the samples sink into the sample wells of the gel; and ¥ tracking dyes so that you have a way of estimating how far the samples have travelled through the gel during electrophoresis. The recipe for 6X loading dye is as follows: ¥ 0.25% bromophenol blue (w/v) ¥ 0.25% xylene cyanol (w/v) ¥ 30%...

Lab 9 – Molecular Biology In this lab, you will prepare an agarose gel and use...

Lab 9 – Molecular Biology In this lab, you will prepare an agarose gel and use gel electrophoresis to compare the size of 2 dye molecules Methyl orange and Ponceau G. You will also analyze an “unknown” sample that contains a mixture of two dyes. Dye molecules with lower molecular weight or greater electrical charge will migrate faster through the gel, than dye molecules with greater molecular weights or lesser electrical charge. Materials: Mini gel electrophoresis chamber 6 Tooth comb...

What amount of agarose (g) and TAE buffer (mL) would you need to make a 1%...

What amount of agarose (g) and TAE buffer (mL) would you need to make a 1% gel?

1X TAE buffer is commonly used as a buffer for DNA gel electrophoresis. You will preform...

1X TAE buffer is commonly used as a buffer for DNA gel electrophoresis. You will preform the calculations necessary to prepare a 50X concentrated stock to store and use throughout the semester. The composition of a 50X TAE stock buffer is 2 M Tris, 1 M acetic acid, 50 mM EDTA, pH 8. Determine how much of each component you will need to make 100 ml of a 50X stock buffer. Show your calculations and construct a table which contains...

Please answer 4 post lab questions thank you Reagents, Supplies and Equipment 1X Blotting buffer pH...

Please answer 4 post lab questions thank you Reagents, Supplies and Equipment 1X Blotting buffer pH 8.3 (25 mM Tris, 192 mM Glycine, 20% ethanol) 1X Blocking buffer (5% nonfat dried milk powder in 1X PBS and 0.025% Tween 20) Wash buffer (1X PBS and 0.025% Tween 20) Nitrocellulose membrane Blotting paper Fiber pads Western Blotting cassette Primary antibody – specifically bind only to myosin light chain protein Secondary antibody HRP color detection substrate (4-chloro-1-naphthol (4CN)) Mini-PROTEAN Tetra gel electrophoresis...

After your frustration with tissue culture, you finally get your cells passaged and decide to set...

After your frustration with tissue culture, you finally get your cells passaged and decide to set up your cDNA synthesis reaction, PCR, and agarose gel. You have extracted RNA from your cells, and now you need to proceed with the cDNA synthesis. The first step is to determine the concentration of your RNA. You dilute your RNA 1:250, vortex it, move it to the cuvette, and run it on the spectrophotometer.   The spec tells you that your concentration of RNA...