Abstract

Leishmaniasis is a major health problem that affects populations of ∼90 countries worldwide, with no vaccine and only a few moderately effective drugs. Here we report the structure/function characterization of sterol 14α-demethylase (CYP51) from Leishmania infantum. The enzyme catalyzes removal of the 14α-methyl group from sterol precursors. The reaction is essential for membrane biogenesis and therefore has great potential to become a target for antileishmanial chemotherapy. Although L. infantum CYP51 prefers C4-monomethylated sterol substrates such as C4-norlanosterol and obtusifoliol (V(max) of ∼10 and 8 min(-1), respectively), it is also found to 14α-demethylate C4-dimethylated lanosterol (V(max) = 0.9 min(-1)) and C4-desmethylated 14α-methylzymosterol (V(max) = 1.9 min(-1)). Binding parameters with six sterols were tested, with K(d) values ranging from 0.25 to 1.4 μM. Thus, L. infantum CYP51 is the first example of a plant-like sterol 14α-demethylase, where requirements toward the composition of the C4 atom substituents are not strict, indicative of possible branching in the postsqualene portion of sterol biosynthesis in the parasite. Comparative analysis of three CYP51 substrate binding cavities (Trypanosoma brucei, Trypanosoma cruzi, and L. infantum) suggests that substrate preferences of plant- and fungal-like protozoan CYP51s largely depend on the differences in the enzyme active site topology. These minor structural differences are also likely to underlie CYP51 catalytic rates and drug susceptibility and can be used to design potent and specific inhibitors.

Highlights

  • Leishmaniasis is widespread on all populated continents: 12 million people in 88 countries are reported to be infected, with 1–2 million new cases and 60,000 deaths occurring each year

  • CYP51 sequences from five Leishmania species are available, and amino acid identities to that from L. infantum are: 95% in L. braziliensis, 96% in L. major, and 97% in L. mexicana and Leishmania amazonensis

  • Accumulation of the CYP51 reaction intermediates in vitro is mostly known as a result of nonoptimal reaction conditions that were used in the experiments to elucidate the reaction mechanism [45, 46]

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Summary

EXPERIMENTAL PROCEDURES

CYP51 Gene Identification, Cloning, and Expression—Sequence data for the L. infantum genome was from the GeneDB website. Cytochrome P450 concentration was determined from the absolute absorbance of the Soret band, using ⑀417 ϭ 117 mMϪ1 cmϪ1 for the low spin ferric form of the protein [16] and . Substrate binding was monitored as a difference type I spectral response reflecting low to high spin transition of the P450 heme iron (blue shift in the Soret band maximum from 417.5 to 393 nm). The apparent dissociation constants (Kd) of the enzyme-substrate complex were calculated by plotting the absorbance changes in the difference spectra (⌬A390–420) upon titration against free ligand concentration and fitting the data to a rectangular hyperbola in Sigma plot statistics.

RESULTS
Secondary structural elementsa
Vmax expb
DISCUSSION

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