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Instrumentation.

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Presentation on theme: "Instrumentation."— Presentation transcript:

1 Instrumentation

2 Chromatography

3 Chromatography Chromatography is the collective term for a set of laboratory techniques for the separation of mixtures. It involves passing a mixture dissolved in a "mobile phase" through a stationary phase, which separates the analyte to be measured from other molecules in the mixture based on differential partitioning between the mobile and stationary phases.

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8 Paper Chromatography Chromatogram of 10 essential oils coloured with vanillin reagent.

9 Development of Chromatogram

10 Paper Chromatography

11 Paper Chromatography Principle Uses Processes
Different components of the mixture have different interactions with the mobile phase and stationary phase so the different components of mixture will travel different distances along the paper. This separates the components of the mixture. Processes Add solvent (mobile phase) to chromatography tank Apply spot of mixture to chromatography paper Dry Place in chromatography tank so that spot is just above mobile phase. Components of mixture separate out as the mobile phase moves up through the paper Uses Separates Coloured Substances

12 Thin Layer Chromatography

13 Thin Layer Chromatography

14 Thin Layer Chromatography
Principle Different components of the mixture have different interactions in the mobile phase and the stationary phase (a thin layer of silica on the glass plate) so the different components will travel different distances along the silica. This separates the components of the mixture. Processes Add solvent (mobile phase) to chromatography tank Apply spot of mixture to TLC plate Dry Place in chromatography tank so that spot is just above mobile phase. Components of mixture separate out as the mobile phase moves up along the TLC plate Uses Separation of dyes taken from fibres in forensic work

15 Column Chromatography

16 Gas Chromatography

17 Gas Chromatography

18 Gas Chromatography

19 This separates the components of the mixture.
Gas Chromatography Principle Different components of the mixture have different interactions with the stationary phase (liquid supported on a porous bed inside a long coiled column) and mobile phase (inert gas for example nitrogen or argon).The different components will travel at different speeds along the column. This separates the components of the mixture. Processes Injection Transport of the sample along the column Separation in the column Detection Uses Drug tests on athletes Blood alcohol tests

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21 High Performance Liquid Chromatography

22 High Performance Liquid Chromatography

23 High Performance Liquid Chromatography (HPLC)

24 High Performance Liquid Chromatography (HPLC)
Principle Different components of the mixture have different tendencies to absorb onto very fine particles of a solid in the HPLC column Solvent that is pumped under pressure through column so the different components will travel different speeds along the column. This separates the components of the mixture. Processes Injection Transport of the sample along the column Separation in the column Detection Uses Growth promoters in meat Vitamins in food

25 HPLC of a mixture of compounds

26 All chromatography needs:
support material – stationary phase solvent (or carrier gas) – mobile phase.

27 Spectroscopy Spectroscopy is analysis of the interaction between electromagnetic radiation and matter. Different types of radiation interact in characteristic ways with different samples of matter The interaction is often unique and serves as a diagnostic "fingerprint" for the presence of a particular material in a sample Spectroscopy is also a sensitive quantitative technique that can determine trace concentrations of substances.

28 Mass Spectrometry Gas Sample Enters Here Filament current Ionises the Gas Ions accelerate towards charged slit Magnetic Field deflects lightest ions most Ions separated by mass expose film

29 Mass Spectrometry

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31 Mass Spectrometry Principle Uses Processes
Positively charged ions are separated on the basis of their relative masses as they move in a magnetic field Uses Identify compounds e.g. in analysis of gases from waste dumps in trace organic pollutants in water in drug testing Measure relative atomic mass Measure relative abundance of isotopes Processes Vaporisation Ionisation Acceleration Separation Detection

32 Mass Spectrometry

33 Atomic Weights and Mass Spectra

34 GC-MS Chromatography Gas chromatography-mass spectrometry (GC-MS) is a method that combines the features of gas-liquid chromatography and mass spectrometry to identify different substances within a test sample. Applications of GC-MS include drug detection environmental analysis identification of unknown samples.

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36 Infra Red Absorption Spectrometry

37 Infra Red Absorption Spectrometry

38 Infra Red Absorption Spectrometry
IR Source Sample Reference Splitter Detector Processor Printout

39 Absorptions of Bonds in Organic Molecules

40 Infra Red Absorption Spectrometry

41 Infra Red Absorption Spectrometry

42 IR of Methanol

43 Infra Red Absorption Spectrometry

44 Infra Red Absorption Spectrometry
Principle Molecules of a substance absorb infra red light of different frequencies. The infra red radiation is absorbed by vibrations of the bonds in the molecules. The combination of frequencies absorbed is peculiar to the molecules of that substance (fingerprinting technique). Processes Infra red radiation passes through the sample The sample absorbs infrared radiation at specific wavelengths which are detected Absorption spectrum is produced Uses Identification of compounds e.g. in Plastics Drugs

45 Ultraviolet-visible spectroscopy

46 Ultraviolet-visible spectrophotomer

47 Ultraviolet Absorption Spectrometry

48 Ultraviolet Absorption Spectrometry
Principle Absorption of ultraviolet radiation by molecules results in the promotion of electrons from their ground state energy levels to higher energy levels Absorbance is directly proportional to concentration Uses Quantitative determination of organic compounds Drug metabolites Plant pigments Processes Ultraviolet light is passed through the sample and a blank The sample absorbs ultra violet radiation at specific wavelengths which are detected Absorption spectrum is produced

49 UV of Benzene

50 Spectra Continuous Spectra Line Spectra Emission Spectra
Absorption Spectra

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52 Emission Spectra

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54 Atomic Absorption

55 Atomic Absorption Spectra
Hydrogen Helium Lithium

56 Energy Staircase Diagram for Atomic Hydrogen
bottom step is called the ground state higher steps are called excited states Summary: line spectra arise from transitions between discrete (quantized) energy states

57 Atomic Absorption Spectrometry

58 Atomic Absorption Spectrometry

59 Atomic Absorption (Magnesium in Water)

60 Atomic Absorption (Lead in Petrol)

61 Atomic Absorption Spectrometry

62 Atomic Absorption Spectrophotometer
Principle Atoms in the ground state absorb light of a particular radiation characteristic of an element. Absorbance is directly proportional to concentration Processes Sample solution is sprayed into the flame, and the sample element is converted into atoms in the element. Ground state atoms absorb radiation from a source made from the element Absorption spectrum is produced Uses Identification of elements Concentration of elements Analysis of heavy metals in water e.g. lead, cadmium

63 Colorimetry A colorimeter is a device used to test the concentration of a solution by measuring its absorbance of a specific wavelength of light. To use this device, different solutions must be made, and a control (usually a mixture of distilled water and another solution) is first filled into a cuvette and placed inside a colorimeter to calibrate the machine. Only after the device has been calibrated can you use it to find the densities and/or concentrations of the other solutions. Wavelength selection Printer button, Concentration factor adjustment Lamp Readout Sample compartment Zero control (100% T), Sensitivity switch.

64 Colorimetry Filter or Diffraction grating to select appropriate beam of light

65 Colorimetry

66 Colorimetry Principle
If a solution is coloured then the intensity of the colour is proportional to the concentration. 2. The percentage of light absorbed by the coloured solution in the colorimeter is proportional to the concentration. Processes Light of a particular wavelength is passed through a number of samples of known concentration. A graph of absorbance against concentration is plotted The absorbance of the unknown is noted and using the graph the concentration of the unknown can be found Uses Analysis Lead in water Fertilisers in water e.g. nitrates and phosphates

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68 Spectra Websites


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