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Transcript
Oct 23, 2006 Handout Answers to Student Questions 1. What happens when a base pair gets deleted? a. If it is in a non-coding region, usually nothing. If it is in a coding region it will cause a frameshift: because codons are made of three nucleotides, deleting one base pair disrupts the “reading frame” or division of the sequence into threes. Frameshifts occur if the number of base pairs inserted or deleted is NOT a multiple of three (if three basepairs are inserted or deleted it will add or delete an amino acid but the reading frame will stay the same). Frameshift mutations are usually highly disruptive and cause proteins to be non-functional. 2. Do all genes have only 2 alleles? a. No. This is known as multiple allelism. Most genes have tens of alleles present in the population. For an example we have discussed in class, blood type in humans has 3 alleles. 3. Do outcomes of certain genotypes sometimes depend on a combination of other preset genotypes? a. By outcomes, if you mean phenotypes, the answer is yes. Some traits are due to a combination of genes and genotypes. For example, eye color. Eye color is not only dependent on the expression of multiple eye color genes, but how dark or light the colors are depends on the amount of melanin or pigment you have. For more on eye color (including banded eye patterns and how is one eye brown and one eye green) read: www.answers.com/topic/eye-color 4. Does co-dominance only work for blood types? a. No. Example: pigment colors in orchids 5. Did Mendel know about co-dominance and incomplete dominance? a. He seems to have known about incomplete dominance (with flowering time). Some people list the “Principle of Incomplete Dominance” as one of his main principles of discovery, but it’s not commonly attributed to him. Sequencing Why do we need to sequence DNA? The Sanger Method/Chain Termination Method 1977 1. Four reaction tubes: From: http://openwetware.org/images/thumb/b/be/Be109dideoxynucleotide.jpg/500pxBe109dideoxynucleotide.jpg 2. From http://www.zerobio.com/sanger1.jpg Dye Terminator Method Mito Lab – PCR visualization by gel electrophoresis Ladder 172 160 166 163 167 177 173 Ladder 500bp- Chem E 355 Aut 06 182 159 164 175 170 168 171 500bp- Ladder 161 162 500bp- Ladder 500bp- 181 178 176 180 177 Ladder 500bp- 169 190 174 10-11-06 ChmE355/599 Transcription? Z O O O O P P P P Y A Low Glucose High Lactose O High Glucose Low Lactose Z Y A Z Y A Low Glucose Low Lactose Z Y A High Glucose High Lactose O O O ChmE355/599 HOMEWORK DUE MON 10-30-06 Regulation The trp operon. A group of genes whose enzymes synthesize the amino acid, tryptophan are clustered together in the “trp operon.” These genes are transcribed when tryptophan levels are low in the cell, i.e., when more tryptophan is needed. They are not transcribed when tryptophan levels are high. 1.Based on the example of the lac operon, how do you think the trp operon might be designed? (Hint: tryptophan is used continuously used by the cell so would the cell likely have the operon continuously “turned on” or “turned off?”). 2. In class we’ve discussed how transcription can be controlled by transcription factors (activators and repressors). Now think about what other potential control points exist. Use the following example. In response to an environmental change, the bacterium Escherichia coli alters the concentration of a particular protein (let’s call this hypothetical protein, Protein X) over the course of a couple of hours. Which of the following are reasonable (theoretically plausible) mechanisms by which the cell could change its concentration of Protein X without affecting the concentrations of other proteins. Specifically, could the cell… A. Alter the sequence of the gene encoding for Protein X? B. Alter the concentration of RNA polymerase in the cell? C. Alter the concentration of nucleotides (NTPs) in the cell? D. Alter RNA polymerase’s access to the promoter of the gene encoding/coding for Protein X? E. Alter RNA polymerase’s ability to move forward along the gene coding for Protein X? F. Alter the rate at which the mRNA coding for Protein X is degraded? G. Alter the concentration of ribosomes in the cell? H. Alter the ribosomes’ access to the ribosome binding site of the mRNA coding for Protein X? I. Alter the concentration of tRNA in the cell? J. Alter the rate at which protein P is degraded? 3. In terms of energy and materials, what do you think would be the most “economical” way for the cell to decrease the concentration of Protein X? Why? 4. What would be the quickest way to decrease the concentration of protein P? Why?
