Literature DB >> 19954434

Synthesis, properties, and applications of diazotrifluropropanoyl-containing photoactive analogs of farnesyl diphosphate containing modified linkages for enhanced stability.

Marisa L Hovlid1, Rebecca L Edelstein, Olivier Henry, Joshua Ochocki, Amanda DeGraw, Stepan Lenevich, Trista Talbot, Victor G Young, Alan W Hruza, Fernando Lopez-Gallego, Nicholas P Labello, Corey L Strickland, Claudia Schmidt-Dannert, Mark D Distefano.   

Abstract

Photoactive analogs of farnesyl diphosphate (FPP) are useful probes in studies of enzymes that employ this molecule as a substrate. Here, we describe the preparation and properties of two new FPP analogs that contain diazotrifluoropropanoyl photophores linked to geranyl diphosphate via amide or ester linkages. The amide-linked analog (3) was synthesized in 32P-labeled form from geraniol in seven steps. Experiments with Saccharomyces cerevisiae protein farnesyltransferase (ScPFTase) showed that 3 is an alternative substrate for the enzyme. Photolysis experiments with [(32)P]3 demonstrate that this compound labels the beta-subunits of both farnesyltransferase and geranylgeranyltransferase (types 1 and 2). However, the amide-linked probe 3 undergoes a rearrangement to a photochemically unreactive isomeric triazolone upon long term storage making it inconvenient to use. To address this stability issue, the ester-linked analog 4 was prepared in six steps from geraniol. Computational analysis and X-ray crystallographic studies suggest that 4 binds to protein farnesyl transferase (PFTase) in a similar fashion as FPP. Compound 4 is also an alternative substrate for PFTase, and a 32P-labeled form selectively photocrosslinks the beta-subunit of ScPFTase as well as E. coli farnesyldiphosphate synthase and a germacrene-producing sesquiterpene synthase from Nostoc sp. strain PCC7120 (a cyanobacterial source). Finally, nearly exclusive labeling of ScPFTase in crude E. coli extract was observed, suggesting that [32P]4 manifests significant selectivity and should hence be useful for identifying novel FPP-utilizing enzymes in crude protein preparations.

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Year:  2010        PMID: 19954434      PMCID: PMC2836812          DOI: 10.1111/j.1747-0285.2009.00914.x

Source DB:  PubMed          Journal:  Chem Biol Drug Des        ISSN: 1747-0277            Impact factor:   2.817


  40 in total

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Authors:  H Zhang; M C Seabra; J Deisenhofer
Journal:  Structure       Date:  2000-03-15       Impact factor: 5.006

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Authors:  Sean A Agger; Fernando Lopez-Gallego; Thomas R Hoye; Claudia Schmidt-Dannert
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