Homework Answers
Answer 4a:)
The image contains the bands of the gel. In this gel, each student will get the band of the same size because it is PCR products in which each student would have the same sample.
Answer 4b:)
The PCR process makes copies of the sample. Therefore, each PCR product will have the same size if each student gets the same sample.
Answer 4c:)
The PCR products of Alexandra and Anastasia might have produced by the nonspecific binding of primers. This makes different types of bands.
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II. Amplify the gene of interest using the PCR, verify the PCR products on the gel...
The technological approaches applied for ancient cal approaches applied for ancient DNA study can also be...
The technological approaches applied for ancient cal approaches applied for ancient DNA study can also be used for forensic genetic analysis in Where only microscopic amounts of material are available or the DNA has been severely damaged. Some of these approaches were used in the genetic expertise of the putative remains on the last Russian Emperor Nicholas II Romanov. is historical evidence that Prince Alexey suffered from severe bleeding that is characteristic of philia. It is now known that hemophilia...
You are using PCR to amplify a 300 bp target sequence, a portion of Gene X,...
You are using PCR to amplify a 300 bp target sequence, a portion of Gene X, from human genomic DNA isolated from patients' blood samples. The instructions for this procedure tell you to include Samples A and B, whose contents are listed below, with each batch of patient samples that you run. Ingredients Sample A Sample B 10x PCR Buffer (Tris,KCI,MgCl2,BSA) 5 mL 5 mL H2O 37.8mL 38.8mL dNTP's 3 mL 3 mL Taq DNA polymerase 0.2 mL 0.2 mL...
You’re trying to PCR amplify a gene, but your gel shows that there are two bands...
You’re trying to PCR amplify a gene, but your gel shows that there are two bands instead of only one like you expected. You know for certain that there no homologous genes in the genome from which you’re amplifying, so you assume that the issue must be coming from your primers or PCR conditions. Briefly describe 2 different strategies for solving the problem and how they work.
Two experiments were performed in order to confirm the Beta-glucuronidase gene from E. coli was present...
Two experiments were performed in order to confirm the
Beta-glucuronidase gene from E. coli was present in the pET28a
plasmid. (Lane1) PCR was performed to amplify the
Beta-glucuronidase gene and if the gene was present then a single
band would appear at ~7,300 bp. However, the band appeared to drag
down the gel but stopped ~7,300 bp. What would cause the PCR
product to smear down the gel and does this mean that the
amplification of the PCR product was...
You PCR amplify a 500 bp (base pairs) piece of DNA that has diagnostic value in...
You PCR amplify a 500 bp (base pairs) piece of DNA that has
diagnostic value in determining whether a patient has a mutation
within a specific DNA region. You know that this DNA segment of the
“normal” gene does not include an EcoRI restriction site; but the
mutated DNA segment of the same gene contains an EcoRI restriction
site due to a point mutation at the 100th bp from the 5’ DNA end.
After PCR amplification, you subject your DNA...
Paragraph Styles The technological approaches applied for ancient DNA study can also be used for forensic...
Paragraph Styles The technological approaches applied for ancient DNA study can also be used for forensic genetic analysis in difficult cases where only microscopic amounts of material are available or the DNA has been severely damaged. Some of these approaches were used in the genetic expertise of the putative remains of the family of the last Russian Emperor Nicholas II Romanov. There is historical evidence that Prince Alexey suffered from severe bleeding that is characteristic of hemophilia. It is now...
Question 1. 1 2 3 4 5 6 7 8 Lane Name/Code Ladder 1B | 2B...
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You are using a ChIP assay to study the positioning of a DNA-binding transcription factor (Dbp1p)...
You are using a ChIP assay to study the positioning of a
DNA-binding transcription factor
(Dbp1p) on transcribed genes. You fragment DNA from wild type
cells and immunoprecipitate
Dbp1p with an antibody to it. Then you PCR amplify the DNA
associated with Dbp1p using
different sets of primers for a particular gene (G3PD). One set
of primers was specific for the
TATA box region of this gene, (lane 1) another pair of primers
amplified the 3’ end of the open...
Can someone help me with this homework question on gel electrophoresis? Translocation and deletion 3. You...
Can someone help me with this homework question on gel
electrophoresis?
Translocation and deletion 3. You PCR amplify a 500 bp (base pairs) piece of DNA that has diagnostic value in determining whether a patient has a mutation within a specific DNA region. You know that this DNA segment of the "normal" gene does not include an EcoRI restriction site; but the mutated DNA segment of the same gene contains an EcoRI restriction site due to a point mutation at...
This is for an a 3 unknown I am doing in Microbiology. And I don't quite...
This is for an a 3 unknown I am doing in Microbiology. And I don't quite understand it, if you could please help thanks A. How did you prepare the template DNA? B. Name the gene that we will be sequencing in order to identify the unknown. C. Explain why this region is considered to be the target for identification instead of sequencing the entire genome? D. What is the size (in bp) of target DNA in E. coli? B....
The technological approaches applied for ancient cal approaches applied for ancient DNA study can also be used for forensic genetic analysis in Where only microscopic amounts of material are available or the DNA has been severely damaged. Some of these approaches were used in the genetic expertise of the putative remains on the last Russian Emperor Nicholas II Romanov. is historical evidence that Prince Alexey suffered from severe bleeding that is characteristic of philia. It is now known that hemophilia...
Two experiments were performed in order to confirm the
Beta-glucuronidase gene from E. coli was present in the pET28a
plasmid. (Lane1) PCR was performed to amplify the
Beta-glucuronidase gene and if the gene was present then a single
band would appear at ~7,300 bp. However, the band appeared to drag
down the gel but stopped ~7,300 bp. What would cause the PCR
product to smear down the gel and does this mean that the
amplification of the PCR product was...
You PCR amplify a 500 bp (base pairs) piece of DNA that has
diagnostic value in determining whether a patient has a mutation
within a specific DNA region. You know that this DNA segment of the
“normal” gene does not include an EcoRI restriction site; but the
mutated DNA segment of the same gene contains an EcoRI restriction
site due to a point mutation at the 100th bp from the 5’ DNA end.
After PCR amplification, you subject your DNA...
Paragraph Styles The technological approaches applied for ancient DNA study can also be used for forensic genetic analysis in difficult cases where only microscopic amounts of material are available or the DNA has been severely damaged. Some of these approaches were used in the genetic expertise of the putative remains of the family of the last Russian Emperor Nicholas II Romanov. There is historical evidence that Prince Alexey suffered from severe bleeding that is characteristic of hemophilia. It is now...
Question 1. 1 2 3 4 5 6 7 8 Lane Name/Code Ladder 1B | 2B 2 DNA Sample/Treatment DNA ladder Digest Digest Digest Digest Digest Digest 3B 4B 5B Negative Figure 1: 1% Super buffer agarose gel electrophoresis of restriction digest of the plasmid containing the gdhA gene insert. Based on the information above answer the following questions? 1. What ladder size used? 2. What are the two top bands and bottom bands representing? 3. Explain why the observed...
You are using a ChIP assay to study the positioning of a
DNA-binding transcription factor
(Dbp1p) on transcribed genes. You fragment DNA from wild type
cells and immunoprecipitate
Dbp1p with an antibody to it. Then you PCR amplify the DNA
associated with Dbp1p using
different sets of primers for a particular gene (G3PD). One set
of primers was specific for the
TATA box region of this gene, (lane 1) another pair of primers
amplified the 3’ end of the open...
Can someone help me with this homework question on gel
electrophoresis?
Translocation and deletion 3. You PCR amplify a 500 bp (base pairs) piece of DNA that has diagnostic value in determining whether a patient has a mutation within a specific DNA region. You know that this DNA segment of the "normal" gene does not include an EcoRI restriction site; but the mutated DNA segment of the same gene contains an EcoRI restriction site due to a point mutation at...
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