Homework Answers
1. Usually an uncut vector is circular which faces friction when subjected to electrophoresis which further results strain on the DNA molecule so that the conformation changes to twisted and knotted. Usually 2-3 bands can be seen in an uncut vector depending upon the conformations to which they belong i.e. linear, circular, open. These forms of uncut DNA move at different rates over electrophoresis gel with supercoiled moving at fastest rate. However, when it is subjected to restriction digestion, then the tension/strain is relieved resulting in the appearance of single band over the agarose gel.
2. Uncut DNA during cloning experiments act as a negative control so that we can differentiate if the transformation has happened successfully. In cut DNA two bands would be seen, one for vector and another for insert.
Add Answer to:
RESULTS: Analyzing your data Answer the following questions: 1) How many bands do you see in...
A1 is my DNA, Enzyme 1 BsrB1 P1 is known pBR322 enzyme 1 A2 is my...
A1
is my DNA, Enzyme 1 BsrB1
P1 is known pBR322 enzyme 1
A2 is my dna enzyme 2 RSa1
p2 is known pBR322 enzyme 2
Au is my dna uncut
Pu is know pBR322 uncut
ladder Pu Au P, A, P2 Az HAAAM .. - וור RESULTS: Analyzing your data Tobbul Avdinol Answer the following questions: 1) How many bands do you see in the "uncut" lanes? If there are more than one band can you explain the nature...
can someone explain throughly on how to find a-c??? thanks!!! The following question will provide practice in interpreting and analyzing gel results. 5. You obtained the DNA electrophoresis gel be...
can
someone explain throughly on how to find a-c??? thanks!!!
The following question will provide practice in interpreting and analyzing gel results. 5. You obtained the DNA electrophoresis gel below. Three samples of lambda phage DNA were digested with 3 different restriction enzymes and the digested DNA was applied to the gel in lane 4 and the bands were visualized. The Hind Ill digest was used as a molecular weight standard marker and produced 6 DNA fragments of known size:...
1. If a restriction enzyme cuts a circular plasmid twice, how many fragments would you see...
1. If a restriction enzyme cuts a circular plasmid twice, how many fragments would you see on the gel? 2. How would you estimate the total number of base pairs in a plasmid by looking at the DNA fragments of the digested plasmid on a gel? 3. If a linear 1kb DNA fragment has a restriction site that is located 50 bp from one end of the plasmid, what would you expect to see if the digested and undigested DNA...
The PCR was a success and your target region of 770 bp in length has been...
The PCR was a success and your target region of 770 bp in length has been amplified. You now plan to digest the DNA amplicon with the restriction enzyme Eael, and clone the resulting longest fragment it into the Eael site of the 5 kb plasmid diagrammed below. 770 bp BamHI 1 200 EcoRI 800 EcoRI 4000 1000 5 kb O /1000 2000 2000 Faal You purify your recombinant plasmid from bacterial cells, and run the plasmid (uncut. or not...
Can you answer these questions pleasee: If we performed electrophoretic separation (AGE) of human genomic DNA...
Can you answer these questions
pleasee: If we performed electrophoretic separation (AGE) of human
genomic DNA (buccal swab extraction), and we didn’t perform any
restriction digestion, answer the following:
a)In your opinion, which of the loaded samples has the highest
and lowest concentration of DNA, respectively?
b)Indicate the lanes in which DNA is degraded and explain your
answer.
c)Take a look into the lane “cut Plasmid”. Explain the appearance
of two bands. What kind of a technique was performed on...
Please I need help on questions 1-4 in great detail please Load 15 mu l of...
Please I need help on questions 1-4 in great detail please
Load 15 mu l of the following samples from the above section onto the simple Wells. Seal the wells with agarose and electrophorese until the bromophenol blue in the samples has migrated to within 2 mm of the positive electrode end of the gel. Remove the gels from the unit and stain them as described in Section IV. Measure the distance of the DNA bands (in cm) from the...
help with questions 5 to 10 please PCB 3023L Lab #4 Protocol & Worksheet (30pt) You...
help with questions 5 to 10 please
PCB 3023L Lab #4 Protocol & Worksheet (30pt) You may work in your lab groups durine class. but all written answers must be completed individually in your own words. 1) Using the plasmid map for orientation 1 and the cDNA map as a guide, complete the plasmid map for orientation #2. (4pt) 612 1318 1 - EcoRi EcoRI Xbal ECORV -Xbal- 1662 +Bell EcoRI EcoRV Not FP -- Xhol X 2015 PRSP +...
Use the following depiction of a gel of Hind III fragments to answer the questions: 1...
Use the following depiction of a gel of Hind III fragments to answer the questions: 1 Kb Ladder Possible Hind III Fragments: 1 Kb Ladder Sizes 10,000 8,000 564 bp 8,888 2.0 kb 2.3 kb 11 4.36 kb 4,000 3,000 2,500 2,000 1,500 6.5 kb 9.4 kb 23 kb 1,000 750 500 250 1. Based on the gel results, list the sizes of the chromosome fragments cloned: 2. Based on the gel results, list the sizes of the chromosome fragments...
I need the answers for questions 2 and 3. My DNA ladder is in lane 2...
I
need the answers for questions 2 and 3. My DNA ladder is in lane 2
marked by the yellow arrow. Thanks!
Here is the only other info I have. Thanks!
Part 2: Gel purification and on Gel Slice and PCR Product Preparin modified from TBSci.com instructions for gaan A. Dissolving the Gel Stie Following electrophores, eral DNA band from grand place glice microcentrifuge tube Ib. Use an analytical balance to weigh pelice Rec die 2. Add 500 balance to...
QUESTIONS Answer the following questions in the data section of your lab report: 1. Use the...
QUESTIONS Answer the following questions in the data section of your lab report: 1. Use the experience you gained from doing the experiment to answer the following: A student tested an unknown mixture that might contain any of the ions tested in this ex- periment and made the following observations: a. On the addition of 6M HCI, the solution remained colorless and no bubbles were observed. b. When 0.1M BaCl2 was added to the acidified unknown, a white precipitate was...
A1
is my DNA, Enzyme 1 BsrB1
P1 is known pBR322 enzyme 1
A2 is my dna enzyme 2 RSa1
p2 is known pBR322 enzyme 2
Au is my dna uncut
Pu is know pBR322 uncut
ladder Pu Au P, A, P2 Az HAAAM .. - וור RESULTS: Analyzing your data Tobbul Avdinol Answer the following questions: 1) How many bands do you see in the "uncut" lanes? If there are more than one band can you explain the nature...
can
someone explain throughly on how to find a-c??? thanks!!!
The following question will provide practice in interpreting and analyzing gel results. 5. You obtained the DNA electrophoresis gel below. Three samples of lambda phage DNA were digested with 3 different restriction enzymes and the digested DNA was applied to the gel in lane 4 and the bands were visualized. The Hind Ill digest was used as a molecular weight standard marker and produced 6 DNA fragments of known size:...
The PCR was a success and your target region of 770 bp in length has been amplified. You now plan to digest the DNA amplicon with the restriction enzyme Eael, and clone the resulting longest fragment it into the Eael site of the 5 kb plasmid diagrammed below. 770 bp BamHI 1 200 EcoRI 800 EcoRI 4000 1000 5 kb O /1000 2000 2000 Faal You purify your recombinant plasmid from bacterial cells, and run the plasmid (uncut. or not...
Can you answer these questions
pleasee: If we performed electrophoretic separation (AGE) of human
genomic DNA (buccal swab extraction), and we didn’t perform any
restriction digestion, answer the following:
a)In your opinion, which of the loaded samples has the highest
and lowest concentration of DNA, respectively?
b)Indicate the lanes in which DNA is degraded and explain your
answer.
c)Take a look into the lane “cut Plasmid”. Explain the appearance
of two bands. What kind of a technique was performed on...
Please I need help on questions 1-4 in great detail please
Load 15 mu l of the following samples from the above section onto the simple Wells. Seal the wells with agarose and electrophorese until the bromophenol blue in the samples has migrated to within 2 mm of the positive electrode end of the gel. Remove the gels from the unit and stain them as described in Section IV. Measure the distance of the DNA bands (in cm) from the...
help with questions 5 to 10 please
PCB 3023L Lab #4 Protocol & Worksheet (30pt) You may work in your lab groups durine class. but all written answers must be completed individually in your own words. 1) Using the plasmid map for orientation 1 and the cDNA map as a guide, complete the plasmid map for orientation #2. (4pt) 612 1318 1 - EcoRi EcoRI Xbal ECORV -Xbal- 1662 +Bell EcoRI EcoRV Not FP -- Xhol X 2015 PRSP +...
Use the following depiction of a gel of Hind III fragments to answer the questions: 1 Kb Ladder Possible Hind III Fragments: 1 Kb Ladder Sizes 10,000 8,000 564 bp 8,888 2.0 kb 2.3 kb 11 4.36 kb 4,000 3,000 2,500 2,000 1,500 6.5 kb 9.4 kb 23 kb 1,000 750 500 250 1. Based on the gel results, list the sizes of the chromosome fragments cloned: 2. Based on the gel results, list the sizes of the chromosome fragments...
I
need the answers for questions 2 and 3. My DNA ladder is in lane 2
marked by the yellow arrow. Thanks!
Here is the only other info I have. Thanks!
Part 2: Gel purification and on Gel Slice and PCR Product Preparin modified from TBSci.com instructions for gaan A. Dissolving the Gel Stie Following electrophores, eral DNA band from grand place glice microcentrifuge tube Ib. Use an analytical balance to weigh pelice Rec die 2. Add 500 balance to...
QUESTIONS Answer the following questions in the data section of your lab report: 1. Use the experience you gained from doing the experiment to answer the following: A student tested an unknown mixture that might contain any of the ions tested in this ex- periment and made the following observations: a. On the addition of 6M HCI, the solution remained colorless and no bubbles were observed. b. When 0.1M BaCl2 was added to the acidified unknown, a white precipitate was...
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