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Peculiarities of Crystallization of the Restriction Endonuclease EcoRIINucleases interfere with most standard molecular biology procedures. We have purified and crystallized the restriction endonuclease EcoRII, which belongs to the type II of restriction- modification enzyme, to study the protein crystallization process using a "non standard" macromolecule. A procedure for the purification of EcoRII was developed and 99% pure protein as determined by SDS PAGE electrophoresis obtained. Light scattering experiments were performed to assist in screening protein suitable crystallization conditions. The second virial coefficient was determined as a function of precipitating salt concentration, using sodium chloride, ammonium sulfate, and sodium sulfate. Small (maximum size approximately 0.2 mm) well shaped crystals have been obtained. Larger poorly formed crystals (ca 0.5 mm) have also been obtained, but we have been unable to mount them for diff-raction analysis due to their extreme fragility. Crystallization experiments with PEG have shown that using this precipitant, the best crystals are obtained from slightly over-saturated solutions. Use of higher precipitant concentration leads to dendritic crystal formation. EcoRII is difficult to solubilize and meticulous attention must be paid to the presence of reducing agents.
Document ID
19980236876
Acquisition Source
Marshall Space Flight Center
Document Type
Reprint (Version printed in journal)
Authors
Karpove, Elizaveta
(National Academy of Sciences - National Research Council Huntsville, AL United States)
Pusey, M.arc L.
(NASA Marshall Space Flight Center Huntsville, AL United States)
Date Acquired
August 18, 2013
Publication Date
January 1, 1998
Subject Category
Solid-State Physics
Meeting Information
Meeting: Crystallization of Biological Maromolecules
Location: Granada
Country: Spain
Start Date: May 3, 1998
Distribution Limits
Public
Copyright
Work of the US Gov. Public Use Permitted.

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