GAS CHROMATOGRAPHY ENVE 202 Dr. Aslıhan Kerç.

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GAS CHROMATOGRAPHY ENVE 202 Dr. Aslıhan Kerç

Gas Chromatography (GC)   Gas chromatography is a chromatographic technique that can be used to separate volatile organic compounds. It consists of a flowing mobile phase an injection port a separation column (the stationary phase) an oven a detector.

Principle The organic compounds are separated due to differences in their partitioning behavior between the mobile gas phase and the stationary phase in the column.

Mobile phases are generally inert gases such as helium, argon, or nitrogen. The injection port consists of a rubber septum through which a syringe needle is inserted to inject the sample. The injection port is maintained at a higher temperature than the boiling point of the least volatile component in the sample mixture.

Since the partitioning behavior is dependent on temperature, the separation column is usually contained in a thermostat-controlled oven. Separating components with a wide range of boiling points is accomplished by starting at a low oven temperature and increasing the temperature over time to elute the high-boiling point components.

A gas chromatography oven, open to show a capillary column

GC Columns Packed columns Capillary columns Thin fused-silica. Typically 10-100 m in length and 250 mm inner diameter. St. ph. coated on the inner surface. Provide much higher separation eff. But more easily overloaded by too much sample. Typically a glass or stainless steel coil. 1-5 total length and 5 mm inner diameter. Filled with the st. ph. or a packing coated with the st.ph.

GC Detectors After the components of a mixture are separated using gas chromatography, they must be detected as they exit the GC column. Thermal-conduc. (TCD) and flame ionization (FID) detectors are the two most common detectors on commercial GCs. The others are Atomic-emmision detector (AED) Chemiluminescence detector Electron-capture detector (ECD) Flame-photometric detector (FPD) Mass spectrometer (MS) Photoionization detector (PID)

GC Detectors Cont’d The requirements of a GC detector depend on the separation application. E.g. An analysis may require a detector selective for chlorine containing molecules. Another analysis might require a detector that is non- destructive so that the analyte can be recovered for further spectroscopic analysis. You can not use FID in that case because it destroys the sample totally. TCD on the other hand is non-destructive.

TCD Detector A TCD detector consists of an electrically-heated wire.The temperature of the sensing element depends on the thermal conductivity of the gas flowing around it. Changes in thermal conductivity, such as when organic molecules displace some of the carrier gas, cause a temperature rise in the element which is sensed as a change in resistance. The TCD is not as sensitive as other detectors but it is non-specific and non-destructive.

ECD Detector Uses a radiactive Beta emitter (electrons) to ionize some of the carrier gas and produces a current between a biased pair of electrodes. When an org. mol. that contains electornegative functional gr., such as halojens, phosphorous and nitro groups, pass by the detector, they capture some of the electrons and reduce the current.

FID Detector Consists of a hydrogen/air flame and a collector plate. The eff. from the GC column passes through the flame, shich breaks down org. mol. and produces ions. The ions are collected on a biased electrode and produce an elec. sig. Extremely sensitive, large dynamic range.

MS Detector Uses the difference in mass-to-charge ratio (m/e) of ionized atoms or molecules to separate them from each other. Molecules have distinctive fragmentation patterns that provide structural information to identify structural components. The general operation of a mass spectrometer is: create gas-phase ions separate the ions in space or time based on their mass to charge ratio Measure the quantity of ions of each mass-to-charge ratio.

MS Detector Cont’d The ion separation power of an MS is described by the resolution: R = m/Dm Where m is the ion mass and Dm is the difference in mass between two resolvable peaks in a mass spectrum. E.g., an MS with a resolution of 1000 can resolve an ion with a m/e of 100.0 from an ion with an m/e of 100.1.