User:Dhea Patel/Notebook/Hemoglobin Project/2013/02/13: Difference between revisions

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==Description==
==Description==
*10.5mg mannitol in Tris buffer, solvent: Acetonitrile
*10.8mg p-sorbitol in phosphate buffer, solvent: Acetonitrile
*10.5mg mannitol in tris buffer, solvent: ethyl acetate
*12.1mg p-sorbitol in phosphate buffer, solvent: ethyl acetate
*11.7mg mannitol in tris buffer, solvent: water
*10.0mg p-sorbitol in phosphate buffer, solvent: water
*11.6mg mannitol in  tris buffer, solvent: chloroform
*10.0mg p-sorbitol in phosphate buffer, solvent: chloroform


*Each solvent was used as a blank.
*Each solvent was used as a blank.

Revision as of 07:56, 15 February 2013

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Objective

  • Run UV-vis and Fluorescence on p-sorbitol in phosphate buffer and mannitol in tris buffer samples in either MeOH, acetone, acetonitrile, ethyl acetate, water, or chloroform.

Description

  • 10.5mg mannitol in Tris buffer, solvent: Acetonitrile
  • 10.8mg p-sorbitol in phosphate buffer, solvent: Acetonitrile
  • 10.5mg mannitol in tris buffer, solvent: ethyl acetate
  • 12.1mg p-sorbitol in phosphate buffer, solvent: ethyl acetate
  • 11.7mg mannitol in tris buffer, solvent: water
  • 10.0mg p-sorbitol in phosphate buffer, solvent: water
  • 11.6mg mannitol in tris buffer, solvent: chloroform
  • 10.0mg p-sorbitol in phosphate buffer, solvent: chloroform
  • Each solvent was used as a blank.
  • The data was corrected for the blank and a corrected baseline.
  • UV-vis scanned from 200-800nm