What is a major drawback of performing genome editing with site-specific endonucleases over RNA-guided endonucleases?   Question 25 options:   difficulty in transformation   Necessity of  protein cargo to facilitate the editing   the need to genetically engineer a new endonuclease for each target sequence.   Specificity is not achieved

Human Anatomy & Physiology (11th Edition)
11th Edition
ISBN:9780134580999
Author:Elaine N. Marieb, Katja N. Hoehn
Publisher:Elaine N. Marieb, Katja N. Hoehn
Chapter1: The Human Body: An Orientation
Section: Chapter Questions
Problem 1RQ: The correct sequence of levels forming the structural hierarchy is A. (a) organ, organ system,...
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Question 36

 

Using Sanger sequencing, starting from the sequencing primer, what is the sequence of the DNA sample ?

 

 
Question 36 options:
 

G T A C C C G A A A T C A G G A

 

A G G A C T A A A G C C C A T G

 

G T A C C C G A A T T C A G G A

 

A G C A C T A A A G C C C A T G

Question 25

 
 

What is a major drawback of performing genome editing with site-specific endonucleases over RNA-guided endonucleases?

 
Question 25 options:
 

difficulty in transformation

 

Necessity of  protein cargo to facilitate the editing

 

the need to genetically engineer a new endonuclease for each target sequence.

 

Specificity is not achieved

 
 
 
 
 

Question 23

 
 
 
 
 
 
 
 

What is not true for Sequence tagged site (STS) markers:

 
Question 23 options:
 

cannot be mapped by fluorescence in situ hybridization (FISH)

 

subset of STS markers are known as expressed sequence tag (EST) markers

 

can readily be screened by a PCR assay

 

short DNA sequences that occur at a unique location in the genome

 
 
 
 
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