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TLS Online TPP Program

#Question id: 413

The hydrolysis of ATP has a large negative DG'°; nevertheless it is stable in solution due to:

#Section 2: General Biology

  1. entropy stabilization.

  2. ionization of the phosphates.

  3. resonance stabilization.

  4. the hydrolysis reaction having a large activation energy.

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TLS Online TPP Program

#Question id: 14434

#Section 5: Bioprocess Engineering and Process Biotechnology

the centrifugal separation of biomass of 80um sized cells of density 1.04kgm-3 was carried out in a tubular centrifuge having a diameter of 15cm and rotating at 1200 rev/min. the axis of rotation was 0.8cm, the liquid viscosity was 1.0kgm-3 and 0.013 gcm-ls-1 respectively. centrifuge length is 40cm, what will be the time required for centrifuging 1000 litres of broth? 
TLS Online TPP Program

#Question id: 27353

#Section 7: Recombinant DNA technology and Other Tools in Biotechnology

What is the correct order of steps in the CRISPR process?
TLS Online TPP Program

#Question id: 5250

#Section 3: Genetics, Cellular and Molecular Biology

A researcher would like to map the location of galE and trpA genes in a new species of bacterium that appears to be closely related to E. coli. He decides to use cotransduction, and generatesnappropriate donor and recipient strains. He is disappointed when cotransduction is not seen in his experiement. What is the most reasonable explanation for this situation?
TLS Online TPP Program

#Question id: 13089

#Section 7: Recombinant DNA technology and Other Tools in Biotechnology

To express a yeast gene in E. coli, your task is to design a strategy to insert the yeast gene into the bacterial plasmid. Below is a map of the area of the yeast genome surrounding the gene in which you are interested.

 
The distance between each tick mark placed on the line above is 100 bases in length
Below are the enzymes you can use, with their specific cut sites shown 5’-XXXXXX-3’ 3’-XXXXXX-5’

 
The plasmid is 5,000 bases long and the two farthest restriction enzyme sites are 200 bases apart. The plasmid has an ampicillin resistance gene somewhere on the plasmid distal from the restriction cut sites.
                              
You do the digestion of the insert and the vector and then ligate the two digestions together. You then transform the ligation into bacteria and select for ampicillin resistance. You get three colonies on your transformation plate. You isolate plasmid from each one and cut each plasmid with the enzyme XbaI. You then run your three digestions on an agarose gel and see the following patterns of bands. Describe what each plasmid actually was that was contained in each of the three colonies.
 
What is the Colony 2’s plasmid is;
TLS Online TPP Program

#Question id: 14280

#Section 5: Bioprocess Engineering and Process Biotechnology

In microbial cultivation, the expression for product synthesis