Homocysteine desulphurase from the protozoan trichomonas...

Chemistry: molecular biology and microbiology – Measuring or testing process involving enzymes or... – Involving hydrolase

Reexamination Certificate

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C435S004000, C435S975000, C435S026000, C435S014000, C530S300000, C536S023100, C536S023200, C536S023720

Reexamination Certificate

active

06306618

ABSTRACT:

FIELD OF THE INVENTION
The present invention relates to an assay for determining homocysteine, cysteine, O-acetyl-L-serine and/or methionine levels in a biological sample using a enzyme which catalyses the degradation of homocysteine, cysteine, O-acetyl-L-serine and/or methionine, the enzyme being particularly homocysteine desulphurase; a polynucleotide fragment encoding protozoan homocysteine desulphurase, a recombinant vector comprising such a polynucleotide fragment, a host cell containing said polynucleotide fragment or said recombinant vector, the protozoan homocysteine desulphurase polypeptide, and pharmaceutical compositions comprising recombinant homocysteine desulphurase for use in medicine or veterinary medicine.
BACKGROUND OF THE INVENTION
An elevated level of homocysteine in the blood appears to be an important indicator for many human disease states. Homocysteine is predictive of vascular disease and stroke, Ueland, P. M. (1992) and Kluijtmans L. A. J. et al (1996); is correlated with forms of diabetes and alcoholism, Cravo, M. L. et al (1996); is used to monitor liver and kidney damage, Bostom, A. G. et al (1996) and neural tube defects, Steegers-Theunissen, R. P. N. (1992) and is associated with certain inborn errors of metabolism, Mudd, S. H., (1989).
Homocysteine levels in blood are conventionally determined using high performance liquid chromatography (HPLC) methods, see for example at Poele-Pothoff M. T. B. et al, (1995). However, HPLC methods employ expensive and elaborate machinery, are generally sophisticated and are considered impractical for many routine analyses.
Patent publication WO93/15220 (Cockbain) describes a method for assaying homocysteine in blood using a homocysteine converting enzyme, S-adenosyl homocysteine hydrolase (SAH-hydrolase). SAH-hydrolase catalyses the conversion of homocysteine with a co-substrate, adenosine, to S-adenosyl-homocysteine. It is then possible, by determining the amount of adenosine consumed, to make a correlation with the amount of homocysteine consumed. The amount of homocysteine in a sample is then determined from differences in adenosine concentration. However, such an assay requires the use of two initial substrates (homocysteine and adenosine) and two enzymes, making it relatively complex. It also involves determining a decrease in the concentration of adenosine, which may not be satisfactory.
U.S. Pat. No. 4,940,658 (Allen et al) describes a method for determining sulphydryl amino acids, including homocysteine levels, in samples of body tissues, method of detecting cobalamin and folic acid deficiency using an assay for total homocysteine levels, and methods for distinguishing cobalamin from folic acid deficiency using an assay for total homocysteine levels in conjunction with an assay for methylmalonic acid. The assays comprise combining a sample with a reference standard comprising a known amount of a sulphydryl amino acid to be assayed, labelled with a suitable marker and measuring the relative amounts of labelled and unlabelled sulphydryl amino acid present for each species with a mass spectrometer. As the amount of labelled species is known, it is therefore possible from calculating the ratio of labelled to unlabelled species to determine the amount of sulphydryl amino acid present in the sample.
U.S. Pat. No. 5,438,017 describes a gas chromatography/mass spectrometry method for analysis of sulphydryl amino acids in a sample of body fluid. The assay relies on the use of a labelled reference sulphydryl amino acid, similar to that described in U.S. Pat. No. 4,940,658, but has additional treatment and/or purification steps prior to analysing the sample by gas chromatography/mass spectrometry.
It will be appreciated that similar to HPLC methods, the assays described above which employ gas chromatography/mass spectrometry are generally sophisticated, use expensive and elaborate machinery and are considered impractical for many routine analyses.
SUMMARY
It is an object to the present invention to provide an assay which obviates and/or mitigates at least some of the above disadvantages.
It is a further object of the present invention to provide a recombinant enzyme capable of catalysing the degradation of homocysteine including use in said assay.


REFERENCES:
patent: 4940658 (1990-07-01), Allen et al.
patent: 5690929 (1997-11-01), Lishko et al.
patent: 5715835 (1998-02-01), Lishko et al.
patent: 5885767 (1999-03-01), Rozzell, Jr.
patent: 5985540 (1999-11-01), Tan et al.
patent: 5998191 (1999-12-01), Tan et al.
patent: 6066467 (2000-05-01), Xu et al.
patent: 6140102 (2000-10-01), Tan et al.
patent: WO93/15220 (1993-08-01), None
patent: WO 99/05311 (1999-02-01), None
Erickson P. et al.; Sequence of cDNA for rat cystathionine&ggr;-lyase and comparison of deduced amino acid sequence with relatedEscherichia colienzymes,Biochem. J., 269:335-340 (1990).
Lockwood B. e al.; Purification and characterization of methionine&ggr;-lyase fromTrichomonas vaginalis,Biochem. J. ,279:675-682 (1991).
Lu Y. et al.; Cloning and Nucleotide Sequence of Human Liver cDNA Encoding for Cystahionine&ggr;-Lyase,Biochemical and Biophysical Research Communications, 189(2): 749-758 (1992).
Thong K. et al.; L-Methionine catabolism in trichomonads,Molecular and Biochemical Parasùology, 23:223-231 (1987).
Thong K. et al.; Trichomonad homocysteine desulphurase activity in trichomonads, XP002049553, Paper received Apr. 26, 1985.
Thong K. et al.; Trichomonas Species: Homocysteine Desulphurase and Serine Sulphydrase Activities,Experimental Parasitology, 63:143-151 (1987).

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