Biological Science (7th Edition)
7th Edition
ISBN: 9780134678320
Author: Scott Freeman, Kim Quillin, Lizabeth Allison, Michael Black, Greg Podgorski, Emily Taylor, Jeff Carmichael
Publisher: PEARSON
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Chapter 20, Problem 15PIAT
Summary Introduction
To review:
The way to determine that a homologous gene for blight resistance exists in the human genome.
Introduction:
The homologous genes are the two genes whose DNA sequence is derived from the same origin. The products of these genes may or may not perform the same function.
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Chapter 20 Solutions
Biological Science (7th Edition)
Ch. 20 - Prob. 1TYKCh. 20 - What is a plasmid? a. an organelle found in many...Ch. 20 - CAUTION The human genome size is 3 billion base...Ch. 20 - Prob. 11PIATCh. 20 - Transgenic plants usually contain genes of...Ch. 20 - Prob. 13PIATCh. 20 - 14. PROCESS OF SCIENCE Why was it important to...Ch. 20 - Prob. 15PIATCh. 20 - Prob. 16PIAT
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- Cap, EA1, and Sap are all genes/proteins of interest in this study. For each gene, what gene product is encoded and where is the gene (the literal DNA sequence) located physically in the cell? I need help fimiding this in the artticle and answer as short as possible https://www.ncbi.nlm.nih.gov/pmc/articles/PMC106848/arrow_forwardWhat is a fluorophore? If you wanted to fluorescently label a brain cell, describe one way you could genetically label a brain cell using a transgenic approach and give one way you could genetically label a brain cell using a gene targeting homologous recombination approach.arrow_forwardHow to calculate the recombination rate between the marker and the gene? For example, how to calculate the recombination rate between the D17S74 marker and the breast cancer gene?arrow_forward
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- 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?arrow_forwardMost organisms display a circadian rhythm, a cycling of biological processes that is roughly synchronized with day length. In Drosophila, pupae eclose (emerge as adults after metamorphosis) at dawn. a)Using this knowledge how would screen for Drosophila mutants that have an impaired circadian rhythm? b)In each case, how would you clone the genes you identified by mutation?arrow_forwardDescribe how you would use replica plating of mutagenized, haploid yeast cells to identify temperature-sensitive (ts) mutations in essential genes needed for yeast growth and survival.arrow_forward
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