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Nuclease-detectable binding sites

Ethidium Switches the Nuclease-Detectable Binding Sites of cis-DDP on DNA... [Pg.62]

All our attempts to observe Pt NMR signals from either PtCli " or cis-Pt( NH3)aCl2 bound to reduced cytochrome c or ribo-nuclease A (RNase) have so far failed. These platinum complexes are known to bind to the sulphur atoms of exposed methionines (residues 65 and 29 of Cyt c and RNase respectively) as shown by our previous H NMR studies on RNase (28) and those of Boswell et al on Cyt c (29) and x-ray crystallography. We assume therefore that the resonances are broadened beyond detection via chemical shift anisotropy relaxation. The restriction of Pt mobility on the protein will lead to a large increase in (see CSA equation above). The anisotropy term would also be expected to increase. Scalar coupling to N will also contribute to the increase in linewidths if nitrogen binding sites are involved. [Pg.185]


See other pages where Nuclease-detectable binding sites is mentioned: [Pg.586]    [Pg.43]    [Pg.138]    [Pg.142]    [Pg.67]    [Pg.95]    [Pg.46]    [Pg.77]    [Pg.306]    [Pg.624]    [Pg.13]    [Pg.13]    [Pg.179]    [Pg.6444]    [Pg.170]   


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