HPLC and GC Flashcards

1
Q

how can we determine the content of compound in a sample?

A

we integrate the area under the peak

How well did you know this?
1
Not at all
2
3
4
5
Perfectly
2
Q

how do we integrate the area under the peak?

A

beer lambert law/ must be fully resolved

How well did you know this?
1
Not at all
2
3
4
5
Perfectly
3
Q

how can purity be assigned?

A

as a % of the total peak area- all peaks are integrated ,add all up and put one of interest/ total

How well did you know this?
1
Not at all
2
3
4
5
Perfectly
4
Q

when assigning a purity what does it wrongfully assume?

A

that all the constituents can be detected by UV light

and purity does NOT assign concentration

How well did you know this?
1
Not at all
2
3
4
5
Perfectly
5
Q

how do you externally calibrate?

A

known conc of standards and samples are injected
Linear range should include expected sample concentration
–The peak area is plotted against the concentration and used as a calibration graph

How well did you know this?
1
Not at all
2
3
4
5
Perfectly
6
Q

what are the drawbacks of an external calbirated graph?

A
time consuming method
–Requires analytical standard 
– Available? Cost?
–Matched matrix
–Injection reproducibility
How well did you know this?
1
Not at all
2
3
4
5
Perfectly
7
Q

what is the comparative method?

A

injection of a standard at a known concentration
–Identify the retention time and record peak area : Area(Std)
–Injection of unknown sample
–Record area of peak with the same tR as above: Area(Sample)

How well did you know this?
1
Not at all
2
3
4
5
Perfectly
8
Q

what is the equation for the comparative method?

A

Area(Std) / Conc(Std) = Area(Sample) / Conc(Sample)

How well did you know this?
1
Not at all
2
3
4
5
Perfectly
9
Q

what does the IS account for?

A

Accounts for injection / some sample prep variation

How well did you know this?
1
Not at all
2
3
4
5
Perfectly
10
Q

what are the IS requirements?

A

Chemically + physically similar to the analyte, but not co-elute
•Not be present in the sample
•Not be reactive with the analyte / matrix
•Be chemically pure (analytical grade)

How well did you know this?
1
Not at all
2
3
4
5
Perfectly
11
Q

what compounds is gas chroatography for?

A

volatile compounds ( liquids)

How well did you know this?
1
Not at all
2
3
4
5
Perfectly
12
Q

is GC high or low efficiency? and why?

A

very high efficiency
Low flow resistance = long columns
–No eddy diffusion
–Rapid mass transfer (thin internal film)

How well did you know this?
1
Not at all
2
3
4
5
Perfectly
13
Q

what is GC readily coupled to?

A

Readily coupled to EI-MS systems

How well did you know this?
1
Not at all
2
3
4
5
Perfectly
14
Q

what is separation dependent on in GC?

A

dependant on distribution ratio between stationary phase (internal film coated silica capillary).

How well did you know this?
1
Not at all
2
3
4
5
Perfectly
15
Q

What is the distribution in GC dependent on?

A

distribution ration dependant on volatility (and hence boiling point)

How well did you know this?
1
Not at all
2
3
4
5
Perfectly
16
Q

what does the lowest bp in GC indicate?

A

(highest volatility) = elutes first.

17
Q

what benefits does splitting the sample have in GC?

A

Splitting the sample improves chromatography – avoids overloading

18
Q

is splitting precise?

A

Process of splitting isn’t 100 % precise

•IS can be used to compensate

19
Q

what is headspace GC?

A

Sampling of the “space” above the sample
•Volatile components diffuse into gas phase to form a headspace gas
•Promoted by heating the sample
•Used for residual solvent analysis e.g. left over from organic reaction or purification