Flourescence Spectroscopy

Question 1

Are florescence spectra of molecules ever a mirror image of an absorption spectrum? Why?

Answer 1

Spacings of the energy levels for the first excited state are similar for absorption and fluorescence processes
This implies that the florescence spectra of molecules is near to mirror image of the absorption spectrum, BUT in reality this is only the case for simple molecules

Question 2

Y axis and X axis of fluorescence spectrum?

Answer 2

Y axis = fluorescence emission (arbitrary units)

X axis = wavelength (nm)

Question 3

Do you need to differ things from different machines?

Answer 3

Yes because different machines will have different units

Question 4

Intensity is proportional to…

Answer 4

The amount of photons emitting that the detector picks up

Question 5

Where does the excitation wavelength come into things on the spectra shape)

Answer 5

The shape of this kind of spectrum does NOT depend on which excitation wavelength was used, whereas the intensity of emission does depend on the excitation wavelength

Question 6

What does the excitation spectrum allow for?

Answer 6

Allow/helps identify suitable wavelengths that can be used to excite the fluorophore

Question 7

When is the excitation spectrum equal to the absorption spectrum?

Answer 7

For dilute solutions

It is a plot of intensity of emission as a function of wavelength

Question 8

How fast is fluorescence?

Answer 8

Nano seconds

Question 9

What does the process of luminescence involve?

Answer 9

Excitation: electrons excited to a higher energy state by light absorption

Luminescence: electrons return to ground state and light is then emitted with less energy - some energy is lost

Question 10

How is energy lost when electrons return to the ground state?

Answer 10

Intersystem crossing
Internal conversions
Relaxations from vibrational and rational levels

Question 11

What is a Jablonski diagram?

Answer 11

Energy diagram that describes the process of photon emission

Question 12

How does fluorescence happen again and again and repeat?

Answer 12

Constant S0–>S1–>S0 allows this to happen

Question 13

What is intersystem crossing?

Answer 13

Molecules relax via non-radiative transition to T1

Requires spin orientation to change

Question 14

What is internal conversion?

Answer 14

Radiation-less transition but vibrational levels need to match

Question 15

In fluorescence, how does energy get lost most commonly from relaxation?

Answer 15

Return from excited singlet state to ground state. Does not require change in spin orientation
Lifetime=nano seconds

Question 16

What is phosphorescence

Answer 16

Return from the triplet excited state to the ground state
Requires a change in spin orientation
Usually forbidden but does happen
Longer lifetime than fluorescence- milliseconds rather than nanoseconds
Generally occurs at longer wavelengths than fluorescence because energy difference between S0 and T1 is smaller

Question 17

What is a fluorophore?

Answer 17

A chromophore that can emit fluorescence

Question 18

Describe the excitation process of fluorescence in detail

Amount of time this takes?

Answer 18

Upon light absorption, a chromophorre that was in the lowest vibrational state (V0) of the ground state S0 is excited to some higher vibrational level (e.g. V1 or V2) of the S1 or S2 state
10^-15 seconds

Question 19

Describe the vibrational relaxation process of fluorescence in detail

Answer 19

Non-radiative relaxation takes place until the lowest (relaxed) vibrational level of S1 is reached.
Molecule may undergo conformational change or react with the environment to achieve this

Time: takes 10^-12 seconds

Question 20

Describe the third process of fluorescence in detail, after vibrational relaxations occur

Answer 20

The molecule then relaxes from this lowest vibrational energy level of the excited state S1 to one of the vibrational energy levels of the ground state. In doing so, fluorescence is emitted

Time: 10^-9 secs

Question 21

What are the following: 
S1 
S2
T1
S0

Answer 21

S1 = 1st excited singlet state 
S2 = 2nd excited singlet state 
T1 = 1st excited triplet state 
S0 = ground state

Question 22

What is Stoke’s shift?

Answer 22

Difference between where you apply energy and the maximum peak for emission
I.e.
The difference in wavelength between absorption and emission

Question 23

In Stokes shift, how is some of the absorbed energy lost?

Answer 23

Due to processes that happen in the excited state limetime e.g.

• vibrational relaxation
• collisional quenching
• energy transfer to other molecules (FRET)
• intersystem crossing
• photobleaching

Question 24

In Stokes shift, if some of the energy is lost during the excited state lifetime, what can we deduce about the wavelength of light emitted by fluorescence

Answer 24

The wavelength of light emitted by fluorescence is higher than the light that was absorbed

Question 25

Describe the relationship between:
Speed of light, frequency, wavelength
And
Energy and frequency

Answer 25

c=f(wavelength)

E=hf

Where h= Plank’s constant and c is the speed of light

Question 26

Is it good for Stokes shift to be small or big and why?

Answer 26

The larger the better, because you can detect more sensitively without detecting input radiation (incidence light)
25nm shift is good

Question 27

How do you perform measurement of fluorescence?

Answer 27

Adjust the concentration: 10 to 100 times less concentrated than those used in absorption spectrometry because fluorescence is very sensitive
Transfer solution to a 4-sided cell
Make sure there are no solid particles, as these cause light scattered

Question 28

Ideal absorption of solution to be put in 4-sided cell?

Answer 28

<0.05

Question 29

Is instrument to instrument variation a thing with this kind of measurement?

Answer 29

Yes. It is so significant that intensity from one machine is very different to that of another
Thus fluorescence is measured in arbitrary units and quantitive analysis can only be done by comparing reading with a reference or a calibration curve obtained on the same instrument

Question 30

Advantages of using fluorescence?

Answer 30

• very sensitive (ug to ng, depending on quantum yield)
• higher selectivity than UV-Vis
• relatively inexpensive (more expensive than UV-Vis but less expensive than MS and NMR)
• can be applied in many cases without separation step (e.g. Chromatography)

Question 31

Limitations of fluorescence

Answer 31

• not all drugs are fluorescent
• use of standards normally required in pharmaceutical analysis (arbitrary units)
• changes in conditions can affect fluorescence properties

Question 32

Describe the instrumentation of fluorescence spectroscopy

Answer 32

Lamp or laster (Xe arc lamp or laser)
Excitation Monochromator 
Cell holder (4-sided and clear) 
Emission monochromator (at 90 degrees to excitation one)
Detector

Question 33

Why is the excitation monochromator and the emission monochromator at 90 degrees to each other?

Answer 33

So excitation light doesn’t hit the detector (incident light)
Fluorescence is a glow and goes in all directions

Question 34

In fluorescence spectra, how many times is the sample excited and at what wavelengths?

Answer 34

When recording a fluorescence spectrum, the sample may be excited at a single wavelength (excitation wavelength) and the emission recorded at several wavelengths.

Question 35

What must be considered when there are 2 molecules with different absorption spectra i.e. Mixed fluorophores?

Answer 35

When there are 2 molecules with different absorption spectra, it is important to consider where a fixed wavelength excitation should be placed

Question 36

Describe a method used whereby there are mixed fluorophores

Why is it good?

Answer 36

Excite at different wavelengths

• distinct peaks
• if overlap–> can see both

This method can also be important to minimise fluorescence from impurities by selecting an excitation where impurity cannot absorb light

Question 37

Name the main factors that can affect fluorescence intensity

Answer 37

Inner filter effect
pH
Photobleaching 
Temperature 
Viscosity 
Presence of oxygen 
Structural solvent

Question 38

Describe what photobleaching is and how it occurs

Answer 38

Too much incident radiation can irreversibly degrade the fluorophore and cause loss of fluorescence
This is photobleaching and occurs with lasers

Question 39

How does the presence of oxygen affect fluorescence intensity?

Answer 39

High concentration of oxygen quenches fluorescence through collisions
For example, Copper (Cu2+) ions quench fluorescence by complexation-static quenching

Question 40

How does viscosity and temperature affect the fluorescence intensity?

Answer 40

Viscosity and temperature have opposite effects
As molecules move more freely (low viscosity or high temp) there is more chance of intermolecular collisions (involving solvent molecules) happening.
This causes loss of energy or deactivation of excited state by nn-radioactive means and thus lower fluorescence

Question 41

How does pH affect the fluorescence intensity?

Answer 41

Fluorescent drugs with ionisable groups can be sensitive to pH
Barbiturates only fluoresce in the di-anionic form and phenol fluoresces at pH 7, when it is an anion

Question 42

What is the inner filter affect?

Answer 42

If you plot intensity(y) against concentration (x) the plot forms almost a U-shape. This means at certain intensities, the intensity could be at two different concentrations.

At high concentrations of drug, fluorescence intensity reaches a plateau and as conc increases further, the intensity will decrease due to inner filter effects, in which the ground state molecules absorb (present in abundance) the fluorescence emitted by the excited molecules.
This explains why we dilute the sample as it gives a linear range

Question 43

How is fluorescence used in BP?

Answer 43

Used as a standard for quantitive analysis
Fluorescent light emitted by the substance examined in relation to that emitted by a standard.
Dissolve substance in solvent.
Set excitation wavelength. Measure the intensity of the emitted light at an angle of 90 degrees to the excitation beam.

Question 44

How is the BP method used as a formula?
State the formula that gives the concentration of the solution to be examined
When is this method valid?

Answer 44

Cx=(IxCs/Is)

Where:
Cx = concentration of solution to be examined
Ix= intensity of light emitted by solution to be examined
Cs= concentration of standard solution
Is=intensity of light emitted by standard solution

Method only valid if fluorescence is linear with concentration (i.e. No inner filter affect)

Question 45

Describe the influence of solvent choice on fluorescence

Answer 45

Polar fluorophores are especially sensitive

Interaction with solvent molecules can offer a non-radiative pathway for energy loss

Question 46

Why would you choose Fluorescence over UV?

Answer 46

Example: ethyinylestradiol tablets
UV not good as excipients absorb too and the drug at a low level (mg)
In this assay, use is made of pH affect to correct for background fluorescence from excipients
Addition of NaOH ionises the phenolic group to make it non-fluorescent

Question 47

Affect of rigidity on fluorescence?

Answer 47

Rigidity affects fluorescence e.g. Formation of chelate (BP limit test for aluminium)

Question 48

Effect of substituents that can affect resonance stability changes on fluorescence?

Answer 48

Electron-withdrawing groups lower fluorescence (e.g. COOH, Halide ions, nitro group) while electron-donating groups raise fluoresce (e.g. NH2, OH)

Question 49

What is derivatisation and how is it used in fluorescence spectromtery?

Answer 49

You add something else onto the molecule you are testing
E.g.
-Some drugs can be made to become fluorescent by chemical treatment (e.g. Digitoxin treated with H2SO4 shows strong fluorescence)
-drugs can also be labelled with specific fluorophores that are reactive towards a certain functional group (generally amines, COOH or SH)

Question 50

Protein/peptide drugs contain what fluorescent groups and how do these groups react after protein folding?

Answer 50

Peptide/protein drugs may contain tyrosine and/or tryptophan that are fluorescent.
The fluorescence of such drugs changes on folding/defolding (denaturisation) as a result of solvent access and rigidity change

Question 51

Problem with derivitization of molecules for fluorescence spectroscopy?

Answer 51

Difficult to know how selective the group is and may have to add a separation step