Labs

Question 1

One of the most numerous protein-protein interactions are __

Answer 1

One of the most numerous protein-protein interactions are enzymes

Question 2

How does the configuration of enzyme aid it in it’s function?

Answer 2

Each enzyme has a characteristic three-dimensional (3- D) shape
By their specific configuration, they hold the reactant molecules in close proximity and in the correct orientation for the reaction to occur
Their specificity is also due to their structure

Question 3

What is lactose composed of?

Answer 3

monosaccharides glucose and

galactose

Question 4

Where does lactase function in the body?

Answer 4

Small intestine

Question 5

Describe lactose pathway in the body when lactase activity is low

Answer 5

With low lactase activity in the small intestine, undigested lactose is passed into the colon where bacteria ferment the sugar to hydrogen gas and organic acids.

Question 6

Where is the gene for lactase found?

Answer 6

The gene for the production of lactase is located on chromosome two.

Question 7

How do genomes of lactose intolerant and tolerant people differ? WHat does it allow to conclude?

Answer 7

there does not seem to be any difference in the DNA of individuals with or without lactase activity. Rather the differences
are in the messenger RNA (mRNA), which may indicate that the primary regulation of this enzyme occurs during translation.

Question 8

Describe strip test for lactose

Answer 8

1. Take a 1000 ul of milk sample and place it in a glass test tube + 500ul of Lactase
2. dip the test area of the strip into the sample to test for the presence of free glucose.
3. Remove any excess milk by gently tapping the strip against the side of the test
   tube.
4. Place the test strip on a piece of paper towel and read after 30 seconds.
5. Compare the colour to the chart on the side of the bottle and record the amount of
   free glucose in each sample

Question 9

What are the sugars in rice, soy and cow milks

Answer 9

Cow Lactose
Soy Sucrose
Rice Glucose

Question 10

At what temp does lactase get denatured? pH?

Answer 10

Temp- above 57

pH- above 10 or 12

Question 11

Fats readily dissolve in other fat solvents such as __ or __

Answer 11

Fats readily dissolve in other fat solvents such as hexane or acetone

Question 12

What is saponification

Answer 12

When lipids are hydrolyzed with an alkali such as NaOH, it is split into glycerol and the fatty acid(s). This process is called saponification, and the sodium salt of the fatty acid produced is soap.

Question 13

How can one determine the degree of bond saturation?

Answer 13

one can utilize a halogen solution such as
iodine or bromide. The extent of saturation can be demonstrated by the degree of
decolourization of these solutions after it comes in contact with the lipid.
Each type of lipid can be classified by its iodine number. The more double bonds a fat contains, the more halogen is required; thus, a high iodine number means a high degree of unsaturation. Generally, animal fats
are saturated and vegetable fats are unsaturated.

Question 14

How can one determine the length of a lipid?

Answer 14

Differences in chain length can be distinguished by the differences in intensity of colour due to the absorption of a chemical known as Sudan III. Longer fatty acid chains give more intense and deeper colour.

Question 15

What do you use in saponification number determination experiment?

Answer 15

non-polar solvent (50% isopropanol and 50% hexane)
KOH
phenolphthalein
titrating thing

Question 16

Name monosaccharides

Answer 16

glucose, fructose and galactose

Question 17

Name disaccharides and their constituents

Answer 17

sucrose = glucose + fructose. 
lactose = glucose + galactose. 
maltose  = glucose + glucose.

Question 18

__ and __ are major sources of carbohydrates for humans

Answer 18

Starch and sucrose are major sources of carbohydrates for humans

Question 19

__ is the most common carbohydrate in the human diet

Answer 19

Starch is the most common carbohydrate in the human diet

Question 20

Glycogen synthesis happens mainly in the __.

Answer 20

Glycogen synthesis happens mainly in the liver.

Question 21

Describe 1st step of glycogen synthesis

Answer 21

uradine triphosphate (energy source) is used to convert glucose-1-phosphate to a compound known as UDP-glucose.

Question 22

Describe 2nd step of glycogen synthesis

Answer 22

The enzyme, glycogen synthase uses these UTP glucose monomers to form a chain of
glycogen (α (1→4) glycosidic bond)

Question 23

Describe how does glycogen branching occur

Answer 23

A protein known as glycogenin and a second
enzyme (amylo (α1→4) to (α1→6) transglycosylase is needed to allow for
branching of the glycogen to occur. These
two compounds catalyze a transfer of last
several monomers residues from the nonreducing end of the chain to the C-6
hydroxyl group of a glucose molecule in the middle of the chain. This branching will only occur if a chain contains a sufficient number of residues

Question 24

Describe how does glycogenolysis occur

Answer 24

The enzyme, glycogen phosphorylase, attacks the Pi on the α 1 → 4 linkages between glucose units at one end and second enzyme attacks the branching points

Question 25

Describe benedict’s test

Answer 25

Benedict’s test is used to detect the presence of reducing sugars. Benedict’s is a clear blue solution of mainly copper sulphate.
Solution of benedict + sugar has to be boiled for 3 min
A positive test is the formation of a precipitate within 5 minutes. The colour of the solution should be brick red.

Question 26

Describe bial’s test

Answer 26

Bial’s reagent is used to test for pentoses. It contains orcinol, HCl, and FeCl3. The orcinol forms coloured condensation product. A positive test is indicated by the formation of a bluish product. All other colours indicate a negative
Sugar + reagent have to be in a hot water bath (almost boiling) for 5 minutes.

Question 27

Describe Seilwanoff’s test

Answer 27

Seilwanoff’s test is a test for ketoses. A positive test is the formation of orange to red/red wine colour within 5 minutes without the formation of a precipitate. Sucrose also tests positive with this assay.
Sugar + reagent have to be in a hot water bath (almost boiling) for 4 minutes.

Question 28

Describe what is a Molisch’s test

Answer 28

Molisch’s test is a test for all carbohydrates; however while monosaccharide react quickly to this test, disaccharides and polysaccharides react more slowly. A positive test is seen when a band of purple appears between the interface of the concentrated sulphuric acid and the sugar solution.

Question 29

What’s a reducing sugar?

Answer 29

reducing sugars have either a free aldehyde functional group or a free ketone functional group as part of their molecular structure.

Question 30

How’s molisch test done?

Answer 30

1. In a test tube, place 2 ml. of glucose solution.
2. Add 2 drops of Molisch’s solution.
3. Mix gently
4. VERY SLOWLY add 2 ml of concentrated sulphuric acid but dropper so 2 distinct
   layers form.
5. A positive test is the formation a purple band at the interface of the two solutions.

Question 31

What is DNA gel electrophoresis?

Answer 31

Gel electrophoresis is a technique used for the separation of deoxyribonucleic acid, ribonucleic acid, or proteins using an electric current applied to a gel matrix

Question 32

How are DNA molecules separate in gel electrophoresis?

Answer 32

By placing the molecules in the gel and applying an electric current, the molecules will move through the matrix at different rates, usually based on size. Nucleic acids have a net negative change and move from negative electrodes located near the top of the gel to positive electrodes at the bottom of the gel. Movement is based on charge and size.

Question 33

What is rate of movement ofDNA particles related to

Answer 33

Migration of the fragments in an electrical field move at a rate that is inversely
proportional to the log10 of their size.

Question 34

What is the gel used in electrophoresis?

Answer 34

In most cases the gel is a cross linked polymer whose composition and porosity is chosen based on the specific weight and
composition of the target to be analysed.

Question 35

WHat is agarose?

Answer 35

Agarose is a gel used in electrophoresis
It is a long chain polysaccharide isolated from seaweed. It is heated in a buffer solution and then cooled it forms a matrix (gel) with buffer solution trapped inside. This
gives rise to a porous lattice in the buffer solution which enables nucleic acid molecules to slip through the lattice holes in order to move toward the positive pole. Larger molecules will be slowed down more than smaller molecules as they will be more
easily trapped in the pores while smaller molecules will pass through.

Question 36

What is another factor that can affect the

migration of the nucleic acid beside the size?

Answer 36

conformation (whether the nucleic acid is single or double stranded) and the charge are also important. As a result, a mixture of large and small fragments of nucleic acids that has been run through an agarose gel will be separated by size

Question 37

What is the influence of agarose % concentration?

Answer 37

Agarose concentration can be varied from 0.75 % to 2 %. As the concentration of the gel rises, the pore size changes. Higher percentage gels have smaller pores which retards nucleic acids movement. High percentage gels are excellent for allowing the separation of small fragments of nucleic acid and lower percentage gels are typically used to separate larger fragments.

Question 38

What is a comb?

Answer 38

A “comb” is used to create wells in the gel to allow for the loading of nucleic acids. These wells are small grooves in the gel where the nucleic acid is placed before running the gel to hold it in place. The well size determines how much of the nucleic acid sample can be loaded.

Question 39

what is the most common buffer in gel electrophoresis?

Answer 39

The most common buffer used in gel electrophoresis is Tris Borate EDTA (TBE)

Question 40

Describe Tris Borate EDTA

Answer 40

The Tris maintains a slightly basic condition (pH 7.3). EDTA prevents enzymatic degradation of nucleic acids as it chelates magnesium ions.

Question 41

How does the dye work in Tris Borate EDTA and what is the purpose

Answer 41

The dye moves more quickly than the nucleic acids and allows tracking the movement of the fragments. It is used as an indicator to alert the researcher to turn off Bovine Trypsin
the power on the electrophoresis chamber before the invisible nucleic runs off the end of the gel. The dye also makes the solution more visible, making it easier to work with during the initial phases of preparation and loading.

Question 42

What is a ladder?

Answer 42

It is a solution of known fragment sizes, which is a standard used to compare sizes of unknown nucleic acids. The ladder usually contains regularly spaced sized samplw

Question 43

What is Ethidium bromide used for?

Answer 43

It is commonly used in molecular biology laboratories for visualizing nucleic acids using electrophoresis and other gel-based nucleic acid separation methods.
Ethidium bromide fluoresces when exposed to ultraviolet light and exhibits a vivid red-orange color when bound to nucleic acids. UV-transilluminator are used to visualize the nucleic acid bands after running the gel

Question 44

What is a downside of Ethidium bromide?

Answer 44

Ethidium Bromide however is quite dangerous to use as it is a carcinogen and a
mutagen

Question 45

What is an alternative for Ethidium bromide?

Answer 45

Today, other products can be used such as SafeView™. These dyes were developed to
replace the more toxic Ethidium Bromide because they appear to be non-carcinogenic. However, most of these alternative are quite expensive so many labs still utilize the more toxic dye.

Question 46

Describe DNA base bonding

Answer 46

Cytosine always bonds with Guanine and Adenine always bonds with Thymine

Question 47

Instead of containing _, RNA contains a different base known of __

Answer 47

Instead of containing thymine, RNA contains a different base known of uracil

Question 48

How can gel electrophoresis results be visualized and identified?

Answer 48

Results can be analysed quantitatively by visualizing the gel with UV light and a gel
imaging device. The image is recorded with a computer operated camera, and the intensity of the band or spot of interest is measured and compared against standards or markers loaded on the same gel.The measurement and analysis are mostly done with specialized
software.

Question 49

What is used to make a gel for DNA electrophoresis . Describe the process

Answer 49

1. Weigh out 2.0 g of agarose into a 250mL conical flask.
2. Add 100mL of 1X TAE
3. Heat for around 30s – 1 min in the microwave to melt. Swirl.
4. Add 2 µL of Ethidium Bromide. Swirl
5. Pour the gel into the gel tray when the conical flask is warm. Be very careful to prevent any air bubbles. Use tips to remove bubbles..

Question 50

What is the voltage for gel electrophoresis?

Answer 50

70 -100 V

Question 51

Describe the principle of chromatography

Answer 51

They all have a stationary phase (a solid and/or a liquid supported on a solid) and a mobile phase (a liquid or a gas). The mobile phase flows through the stationary phase and carries the components of the mixture or chemical with it.
Different components travel at different rates.

Question 52

It is important that the solvent level is _ the line with the spots(amino acids) on it

Answer 52

It is important that the solvent level is below the line with the spots(amino acids) on it

Question 53

Describe solvent used for amino acid detection?

Answer 53

solvents are polar binary, ternary or more complex mixtures of water, alcohols, and acids or bases

Question 54

How are amino acids made visible on the paper?

Answer 54

At 100°C, ninhydrin reacts with α-amino acids to form a purple colour, allowing the amino acids to be visualized

Question 55

What is the formula for Rf value?

Answer 55

distance travelled by compound/ distance travelled by solvent

Question 56

How is the distance traveled by a compound measured?

Answer 56

The distance travelled by the compound is measured by measuring from the start line to the middle of the coloured spo