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Spectrofluorimeter

FluoroMate FS-2

 

Fluorescent light or Phosphorescence light measurement

 

Fluorescence is the phenomenon in which absorption of light of a given wavelength by a fluorescent molecule is followed by the emission of light at longer wavelengths. The distribution of wavelength-dependent intensity that causes fluorescence is known as the fluorescence excitation spectrum, and the distribution of wavelength-dependent intensity of emitted energy is known as the fluorescence emission spectrum.

Fluorescence detection has three major advantages over other light-based investigation methods: high sensitivity, high speed, and safety. The point of safety refers to the fact that samples are not affected or destroyed in the process, and no hazardous byproducts are generated.

Sensitivity is an important issue because the fluorescence signal is proportional to the concentration of the substance being investigated. Relatively small changes in ion concentration in living cells can have significant physiological effects. Whereas absorbance measurements can reliably determine concentrations only as low as several tenths of a micromolar, fluorescence techniques can accurately measure concentrations one million times smaller -- pico- and even femtomolar. Quantities less than an attomole (<10-18 mole) may be detected.

Using fluorescence, one can monitor very rapid changes in concentration. Changes in fluorescence intensity on the order of picoseconds can be detected if necessary.
Because it is a non-invasive technique, fluorescence does not interfere with a sample. The excitation light levels required to generate a fluorescence signal are low, reducing the effects of photo-bleaching, and living tissue can be investigated with no adverse effects on its natural physiological behavior.

Configuration of FluoroMate FS-2

The FluoroMate FS-2 is comprised of a Light Source, Excitation and Emission Monochromators & Detectors and the Sample Compartment. The 150W Xenon lamp provides sample illumination over a 200nm ~ 900nm range. The light is split in two by a Beam Splitter located directly in front of the Sample Compartment. One beam irradiates the Sample while the remainder is read by a Photodiode detector, monitoring excitation energy. The light emitted by the Sample is detected by a PMT detector after passing through the Monochromator. To ensure higher emission intensity, we use a specially developed signal amplifying PMT.

Applications

Designed for high precision and accuracy, the FluoroMate FS-2 ensures superior results and reliability for a wide range of applications, including:

  • Life Sciences
    Study of basic biological reactions measuring low volume samples, polarization/anisotropy.

  • Pharmaceuticals and Medicine
    Measuring trace levels of antibiotics, providing information on the structure of nucleic acids, Proteins and viruses.

  • Analytical Chemistry
    Identification and detection of fluorescent material, solvent effect, quantum yields and lifetimes, chemical reactions.

  • Environmental management
    Detection and identification of organic and inorganic toxic substances in air, water and soil.

  • Industry
    Nutritional quality in the food industry. Quality of paint, polymers, optical brighteners and phosphor coatings.  Characterization of crude oils.

  • Photo Chemistry
    Catheterization of excited states, micelle structure, reaction kinetics in micelles.

Specifications

  • Light source: 150W Xenon lamp
  • Wavelength Range: 200 nm ~ 900nm
  • Sensitivity: S/N>500 (peak to peak)
  • Grating: 1200grooves/250 nm blazing (200nm ~ 900nm
  • Wavelength Scan speed: Max. 5000 nm/min
  • Wavelength Drive speed: 10,000 nm/min
  • Wavelength Accuracy: Within +-2nm
  • Wavelength repeatability: Within +-2nm
  • Slit width: variable 1nm, 2nm, 5nm, 10nm, 20nm
  • Dimensions: 518mm(W)×604mm(D)×272mm(H)
  • Weight: 43.7kg
  • Power requirement: 100 ~ 132 VAC 50/60 Hz or 180 ~ 240 VAC 50/60 Hz  (Selectable)

 

 

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