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Keck Home PageNew Services in the Keck Facility

New Services in the Keck Facility

Multiplexed Isobaric Tagging Technology (iTRAQ™)

This new protein profiling service allows researchers to multiplex four samples, providing both identification and quantitation on hundreds to proteins simultaneously.

Affymetrix Microararry Resource at Yale

Opened February 1, 2002 and is now providing all services to both Yale and non-Yale investigators.

HPLC SEC/Laser Light Scattering Determination
of Native Protein Molecular Weights

When coupled with HPLC size exclusion chromatography (SEC), laser light scattering (LS) provides the unique capability of determining the absolute molecular weights of proteins and their protein:protein complexes. More information about the service in Laser Light Scattering  Determination of Native Protein Molecular Weights.

High resolution and high mass accuracy Fourier transform ion
cyclotron resonance (FT-ICR) mass spectrometer

FT-ICR MS offers the highest mass resolving power and highest mass accuracy out of all mass spectrometer types and is ideal for analysis of complex biological sample mixtures. The instrument is used to identify proteins from accurate mass of tryptic digests, to elucidate posttranslational modifications (PTM) of proteins/peptides, to determine exact mass on small molecules, to determine accurate mass of proteins and/or protein mixture, to provide comparative protein profiles in two different proteomes, and to de novo sequence peptides and proteins. When internally calibrated all exact mass measurement accuracies typically fall <2 ppm (parts per million), and all peptide masses, when calibrated externally, used for protein identification fall within <3ppm.

Our 9.4 Tesla Bruker Apex Qe FTMS "Combi" system is equipped with a combination of Matrix assisted laser desorption ionization [MALDI] and conventional and as well as nano Electrospray ionization [ESI] sources. Multiple fragmentation techniques (Collision induced dissociation [CID, MSn], Infrared multiphoton dissociation [IRMPD], and Electron captured dissociation [ECD]) can be selected to enhance determination of post translationally modified sites both in peptides and intact proteins. Contrary to popular belief, the use of various forms of hyphenated techniques (LC-MS, 2DLC-MS, LC-MS/MS, etc.) are now possible with this platform. These various features and the technical capabilities of the FTMS system expand its use for a variety of proteomics applications. Please see detail description of the current services offered with our FTMS system.

 

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Last modified: 20-Dec-2006 (GB)