Applied Biochemical Techniques Flashcards
(41 cards)
explain how a spectrophotometer works and how it can be used to determine concentration of analyte
- light of continuous spectrum emerges from light source
- light passes through prism/grating which splits and refracts light into composite wavelengths
- sample is held in cuvette
- incident light enters into sample ad transmitted light emerges from sample
- intensity of transmitted light is detected by photodetector
- spectrophotometer then calculates amount of monochromatic light absorbed by sample
- intensity of light absorbed can be used to determine concentration of analyte
describe each component parts of a spectrophotometer and the function of each part
light source - provides light that generates a continuous spectrum
cuvette - holds sample
prism/grating - splits and diffracts light into composite wavelengths
photodetector - detects intensity of transmitted light
what is the difference between incident light and transmitted light?
- incident light enters into the sample
- transmitted light emerges from the sample
what is absorbance (A)?
the amount of monochromatic light absorbed by a sample
what is meant by the term λmax?
wavelength of light that is most strongly absorbed by the substance of interest
why is it important to calibrate the spectrophotometer with a blank?
to take into account the natural absorbance of the solvent
how is the effect of pH on the absorption spectra minimised?
prepare the sample in a suitable buffer solution
explain why it is important to control the temperature of the sample during spectrophotometry?
temperature impacts on absorption measurements by causing expansion or contraction of solvent, changes to reaction rates
what are the three factors of Beer-Lambert law that affect how much light is absorbed by a sample?
ϵ = molar absorptivity (how strongly a substance absorbs light of a given wavelength)
l = path length of cuvette (cm) (distance the light travels through the sample)
c = concentration of substance in a sample (moll-1)
state the Beer-Lambert equation
A = ϵlc
explain how you would use absorbance and concentration to determine the concentration of an unknown sample
- create a standard curve by measuring absorbance of known concentrations
use standard curve
- identify absorbance on y axis
- read along to line of best fit and read down to y axis
- mark this on graphs using dotted line
explain a limitation of the Beer-Lambert law
high concentrations
- molecular interactions can take place
- causes changes to the position and shape of absorption bands
- limitation of BL law as it affects linearity of the relationship between sample concentration and absorbance
- low concentrations must be used
state 2 applications of spectrophotometry
- enzyme activity
- quality/quantity of pharmaceuticals
describe the basic principles of ion exchange chromatography
- matrix in column made up of polymer beads with a charge
- molecule mixture added to column and opposite charges attract
- molecules eluted by washing column with increasing concentrations of salt solution (NaCl)
- molecules move through column at rates determined by their charge
explain how sodium chloride can be used to elute during ion exchange chromatography
molecule of interest has negative charge
- chlorine ions compete to bind with the matrix
- molecule with weakest negative charge elutes first
molecule of interest has positive charge
- sodium ions compete to bind with matrix
- molecule with weakest positive charge elutes first
what charge does the column have if it is an ion exchange column?
anions are negative so the column must be positive
what charge does the column have if it is a cation exchange column?
cations are positive so the column must be negative
describe the basic principles of affinity chromatography
- column contains binding ligands that bind to the molecule of interest
- molecule mixture added to column
- target molecule becomes trapped (binds to ligand)
- elute using a ligand solution of higher concentration
what is used for elution during affinity chromatography?
ligand solution (for example substrate)
when separating enzymes using affinity chromatography, what property of the enzyme is being taken advantage of?
that it will bind to a substrate
why does HPLC give a higher resolution compared to low pressure techniques?
sample spends less time in the column
what type of gel is used to separate DNA fragments?
agarose
what type of gel is used to separate proteins?
polyacrylamide
what is the charge at the top of the tan next to the wells during DNA electrophoresis?
negative charge
