A newly developed qPCR has an efficiency of 75%, and each cycle is pretty consistent. In this qPCR, if a reporter and quencher located at the ends of a probe, respectively, are separated far enough from each other, one (1) probe produces a signal of S. Let's assume that we start with only one (1) copy of target dsDNA. How much signals can we obtain after 15 cycles in terms of S if we use the following prob
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A newly developed qPCR has an efficiency of 75%, and each cycle is pretty consistent. In this qPCR, if a reporter and quencher located at the ends of a probe, respectively, are separated far enough from each other, one (1) probe produces a signal of S. Let's assume that we start with only one (1) copy of target dsDNA. How much signals can we obtain after 15 cycles in terms of S if we use the following probes?
(a) Molecular beacon probe
(b) TaqMan probe
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Hello, I still can't understand why we get about 24500 signals. Please let me know what formula I should use.
- T. Miyake and M. Demerec examined proline-requiring mutations in the bacterium Salmonella typhimurium (). On the basis of complementation testing, they found four proline auxotrophs: proA, proB, proC, and proD. To determine whether proA, proB, proC, and proD loci were located close together on the bacterial chromosome, they conducted a transduction experiment. Bacterial strains that were proC+ and had mutations at proA, proB, or proD were used as donors. The donors were infected with bacteriophages, and progeny phages were allowed to infect recipient bacteria with genotype proC− proA+ proB+ proD+. The recipient bacteria werethen plated on a selective medium that allowed only proC+ bacteria to grow. After this, the proC+ transductants were plated on selective media to reveal their genotypes at the other three pro loci. The following results were obtained: Q.Which genotypes represent single transductants and which represent cotransductants?T. Miyake and M. Demerec examined proline-requiring mutations in the bacterium Salmonella typhimurium (). On the basis of complementation testing, they found four proline auxotrophs: proA, proB, proC, and proD. To determine whether proA, proB, proC, and proD loci were located close together on the bacterial chromosome, they conducted a transduction experiment. Bacterial strains that were proC+ and had mutations at proA, proB, or proD were used as donors. The donors were infected with bacteriophages, and progeny phages were allowed to infect recipient bacteria with genotype proC− proA+ proB+ proD+. The recipient bacteria werethen plated on a selective medium that allowed only proC+ bacteria to grow. After this, the proC+ transductants were plated on selective media to reveal their genotypes at the other three pro loci. The following results were obtained: Q.Is there evidence that proA, proB, and proD are located close to proC? Explain your answer.T. Miyake and M. Demerec examined proline-requiring mutations in the bacterium Salmonella typhimurium (). On the basis of complementation testing, they found four proline auxotrophs: proA, proB, proC, and proD. To determine whether proA, proB, proC, and proD loci were located close together on the bacterial chromosome, they conducted a transduction experiment. Bacterial strains that were proC+ and had mutations at proA, proB, or proD were used as donors. The donors were infected with bacteriophages, and progeny phages were allowed to infect recipient bacteria with genotype proC− proA+ proB+ proD+. The recipient bacteria werethen plated on a selective medium that allowed only proC+ bacteria to grow. After this, the proC+ transductants were plated on selective media to reveal their genotypes at the other three pro loci. The following results were obtained: Q.Why are there no proC− genotypes among the transductants?
- DNA from a strain of Bacillus subtilis with the genotype trp+ tyr+ was used to transform a recipient strain with the genotype trp− tyr−. The following numbers of transformed cells were recovered: Genotype Number of transformed cells trp+ tyr− 154 trp− tyr+ 312 trp+ tyr+ 354 What do these results suggest about the linkage of the trp and tyr genes?In a generalized-transduction experiment, phages arecollected from an E. coli donor strain of genotype cys+leu+ thr+ and used to transduce a recipient of genotypecys- leu- thr-. Initially, the treated recipient populationis plated on a minimal medium supplemented with leucine and threonine. Many colonies are obtained.a. What are the possible genotypes of these colonies?b. These colonies are then replica plated onto threedifferent media: (1) minimal plus threonine only, (2)minimal plus leucine only, and (3) minimal. Whatgenotypes could, in theory, grow on these three media?c. Of the original colonies, 56 percent are observed togrow on medium 1, 5 percent on medium 2, and nocolonies on medium 3. What are the actual genotypes ofthe colonies on media 1, 2, and 3?d. Draw a map showing the order of the three genes andwhich of the two outer genes is closer to the middle geneIn 1965, Jon Beckwith and Ethan Signer devised a method of obtaining specialized transducing phages carrying the lac region. They knew that the integration site, designated att80, for the temperate phage φ80 (a relative of phage λ) was located near tonB, a gene that confers resistance to the virulent phage T1: tonB att80 They used an F ′ lac+ plasmid that could not replicate at high temperatures in a strain carrying a deletion of the lac genes. By forcing the cell to remain lac+ at high temperatures, the researchers could select strains in which the plasmid had integrated into the chromosome, thereby allowing the F ′ lac to be maintained at high temperatures. By combining this selection with a simultaneous selection for resistance to T1 phage infection, they found that the only survivors were cells in which the F ′ lac had integrated into the tonB locus, as shown here: tonB F lac att80 This result placed the lac region near the integration site for phage φ80. Describe the subsequent…
- Austin Taylor and Edward Adelberg isolated some new strains of Hfr cells that they then used to map several genes in Escherichia coli by using interrupted conjugation. In one experiment, the researchers mixed cells of Hfr strain AB‑312, which were xyl+ mtl+ mal+ met+ and sensitive to phage T6, with F− strain AB‑531, which was xyl− mtl− mal− met− and resistant to phage T6. The cells were allowed to undergo conjugation. At regular intervals, the researchers removed a sample of cells and interrupted conjugation by killing the Hfr cells with phage T6. The F− cells, which were resistant to phage T6, survived and were then tested for the presence of genes transferred from the Hfr strain. The results of this experiment are shown in the graph. On the basis of these data, give the order of the xyl, mtl, mal, and met genes on the bacterial chromosome and the minimum distances between them in minutes. The origin of transfer is represented by the red triangle. The distances between genes are not…Let’s suppose a new strain of P1 phage has been identified thatpackages larger pieces of the E. coli chromosome. This P1 strainpackages pieces of the E. coli chromosome that are 5 minuteslong. If two genes are 0.7 minute apart along the E. coli chromosome,what would be the cotransduction frequency using a normalstrain of P1 and using the new strain of P1 that packages largerpieces? What would be the experimental advantage of using thisnew P1 strain?Austin Taylor and Edward Adelberg isolated some new strains of Hfr cells that they then used to map several genes in E. coli by using interrupted conjugation . In one experiment, they mixed cells of Hfr strain AB-312, which were xyl+ mtl+ mal+ met+ and sensitive to phage T6, with F− strain AB-531, which was xyl− mtl− mal− met− and resistant to phage T6. The cells were allowed to undergo conjugation. At regular intervals, the researchers removed a sample of cells and interrupted conjugation by killing the Hfr cells with phage T6. The F− cells, which were resistant to phage T6, survivedand were then tested for the presence of genes transferred from the Hfr strain. The results of this experiment are shown in the accompanying graph. On the basis of these data, give the order of the xyl, mtl, mal, and met genes on the bacterial chromosome and indicate the minimum distances between them.
- Would the application of paclitaxel to a cell make us incapable of performing karyotyping on that cell? Why or why not?Why is QTL mapping in human genetic diseases important?If you are using a restriction enzyme that make 8 cuts in the Lambda phage DNA, how many bands (pieces) do you expect to be generated assuming each band is a unique size?