You have isolated a sample of liver cells before a meal and after a meal. You...

1. You have cloned the gene sequence of the novel eukaryotic protein you have named Protein...

1. You have cloned the gene sequence of the novel eukaryotic protein you have named Protein Bob (2,100 bpin length). You have used PCR to amplify up the Protein Bob gene from your isolated genomic DNA. After growing up colonies and testing the plasmid you discovered that your cloning protocol has gone according to plan and you did every step correctly, there was no human error. Yet, there is no functional protein production. Explain the reasoning behind this problem. How...

After decades of work, an old classmate of yours has isolated a small amount of attractase,...

After decades of work, an old classmate of yours has isolated a small amount of attractase, an enzyme producing a powerful human pheromone, from hair samples of Hollywood celebrities. To produce attractase for his personal use, he isolated the human attractase gene directly from a human genomic DNA library. Your friend then inserted the gene into a bacterial expression vector and then introduced the recombinant plasmid into an appropriate E. coli strain for expression of the protein with a fusion...

You perform a real time qPCR experiment using mRNA isolated from HCT116 colon cancer cells grown...

You perform a real time qPCR experiment using mRNA isolated from HCT116 colon cancer cells grown in controlled atmosphere incubators at 0.5% or 16% O2. You want to determine relative expression levels of the HIF1α response gene pyruvate dyhydrogenase kinase (PDHK). For sample one, the reaction takes 21 cycles to enter exponential phase and cross the cycle threshold. Sample 2 takes 26 cycles. Reactions amplifying β-tubulin as a loading control from samples 1 and 2 both took 22 cycles to...

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...

1) You have two unknown, unlabeled clear solutions. One is DNA and the other is protein....

1) You have two unknown, unlabeled clear solutions. One is DNA and the other is protein. How do you determine which solution is DNA, which one is protein 2)In an SDS gel larger proteins travel ________________(longer/shorter) distance compared to smaller proteins. 3) Assuming that the isolation and purification of Rubisco went as expected, which fraction isolated should have the highest concentration of pure Rubisco? Please explain. (There was a total of 11 fractions) 4) Your first task as a graduate...

1. After treating some cells with a compound and examining the mRNA levels and the protein...

1. After treating some cells with a compound and examining the mRNA levels and the protein levels in the cell, what is a possible reason that mRNA levels and protein levels won't coincide? A. The promoter is turned on more. B. The mRNA transcripts degradation is being inhibited. C. Protein levels equal mRNA levels. D. None of the above 2. Which of the following is different between prokaryotes and eukaryotes? A.Prokaryotes are polycistronic and eukaryotes are monocistronic B. Prokaryotes have...

Control of Gene Expression 1. How is it possible that individual cells of a multicellular organisms,...

Control of Gene Expression 1. How is it possible that individual cells of a multicellular organisms, which contain all the same DNA, can be so different from one another? 2. What are housekeeping proteins? What are their roles in the cell? 3. Describe the ways in which cells control gene expression. 4. How does control of transcription in prokaryotes and eukaryotes differ? 5. What is the role of operons in the prokaryotic genome? 6. A rare mutation occurs in bacteria...

1) In most laboratory applications, for plate counts to be considered valid, they must have between...

1) In most laboratory applications, for plate counts to be considered valid, they must have between 30 and 300 colony forming units on them. To achieve this, scientists must dilute the sample prior to plating it. If a culture of bacteria is experiencing exponential growth has 8,449 cells per mL, and an instantaneous growth rate constant of 0.5 hours-1, after 2 hours, what is the total dilution that needs to be performed to yield 71 colony forming units on an...

Genetic code backwards: You have just discovered a small neuropeptide that makes your friend have "dancing...

Genetic code backwards: You have just discovered a small neuropeptide that makes your friend have "dancing feet". Whenever they hear a certain song, they just have to dance. As fun as it is to make them dance whenever you want, you realize that this could be a serious problem and want to help. Since you do not have "dancing feet", you have a normal neuropetide.   You both go to a research clinic and have the small neuropetide sequenced. Your normal...

1. After re-do your culture, you now have to amplify your report gene so that you...

1. After re-do your culture, you now have to amplify your report gene so that you have enough DNA to continue your experiment. You decided to alter the concentration of template DNA strand as a testing condition. After PCR, you decided to run a gel electrophoresis to see the results of your testing condition. You loaded your ladder and enough DNA to give you bands that are bright enough to visualize. However, after you run the gel and take it...