-ELSD.pptx

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Transcript -ELSD.pptx 

EVAPORATIVE LIGHT
SCATTERING DETECTOR
(ELSD)
ANALATYCAL CHEMISTRY
427 PHC
Done by:
Madawi AlUbied
Areej Alsuwayyid
OBJECTIVES
1. What is Evaporative Light Scattering Detector ?
2. Capabilities
3. how does it work?
4. Characteristic properties
5.
Advantages
6. Sensitivity
7. Problems
1. WHAT IS EVAPORATIVE
LIGHT SCATTERING
DETECTOR ?
• Evaporative Light Scattering
Detectors (ELS Detectors) are
essentially universal detectors.
• primarily used in High Performance
Liquid Chromatography (HPLC).
• ELS detectors are an ideal substitute,
or supplement to, traditional HPLC
detectors for liquid chromatography
concentration detection.
2. CAPABILITIES
• The detector responds to all compounds that are, relative to their
mobile phase, sufficiently nonvolatile at the conditions of analysis.
• ELSD is suitable for all LC separated analyses that does not have
light absorbing chromophores.
So it dose not rely on optical properties .
Ex:
phospholipids, carbohydrates, amino acids , fatty acids and
synthetic polymers.
3. HOW DOES IT WORK?
3 key stages:
2
3
1
STAGE 2: EVAPORATION
4. CHARACTERISTIC PROPERTIES
I.
Low background noise (no solvent peaks)
II. Reproducibility (in the 1μg range, STD ~ 1%)
III. Low band broadening (short transit time)
IV. “Near” linear response (instrument and
concentration dependent, smart choice of stand)
5. ADVANTAGES
1. No sample preparation
2. No drivatisation
3. Universal - responds to all compounds in the mobile phase
4. Not dependent on spectroscopic properties of analyte
5. Not susceptible to baseline drift during gradient elution,
temperature or solvent pump fluctuations
6. ELSD compatible with a much wider range of solvents compared
to Refractive Index detector
7. No interference from solvent front peaks (enables fast analysis)
8. Flow rates up to up to 5ml/min can be achieved with no affect on
baseline stability
9. Ideal for High Throughput Screening and quantification
THE ELSD IMPROVES BASELINE STABILITY
AND DETECTION SENSITIVITY COMPARED
TO RI
10278
1. Fructose
2. Glucose
3. Sucrose
1027
7
Column:
Prevail™ Carbohydrate ES, 5µm,
53 x 7mm (Part No. 35104)
Acetonitrile:Water (75:25)
2.0mL/min
Mobile Phase:
Flowrate:
RI
ELSD
6. SENSITIVITY
Sensitivity with ELSD is limited to 1–50 ng on-column in the
best instances.
the followings factors are considered to be affect ELSD
sensitivity :
• Gas quality
• Solvent quality
• Column contributions
• Solvent modifiers
7. PROBLEMS:
 arising with an ELSD are usually manifest in a noisy baseline.
This can have several causes:
1. Evaporation Temperature too low: the solvent is not
completely evaporated.
2.
Evaporation Temperature too high: the solvent is boiling
in the nebuliser.
3.
Air or nitrogen not clean: remove traces of water or oil with
a filter.
4. Gas flow too low: poor nebulisation of the eluent.
 Involatile material in the eluent: replace any buffer salt with a
volatile one (such as ammonium acetate) and ensure that the
eluent is particle free.
REFERENCES
• http://www.usedhplc.co.uk/UsedHPLCIntroductiontoEvaporativeLightScatteringDetectorsELSD.htm
• http://www.separationsnow.com/details/ezine/sepspec10174e
zine/Exploring-the-alluring-charms-of-a-charged-aerosoldetector-for-HPLC.html?tzcheck=1
• http://www.laserchrom.com/LaserchromHPLCTechnicalSupportCentre-TechnicalTips-IntrotoELSD.htm
• http://fxg-ent.com/downloads/SoftaELSDBrochure.pdf