Your search keyword '"Saudan C"' showing total 47 results

1. High-Pressure Stopped-Flow Studies to Characterize Transient Conformational Transitions of a Membrane Enzyme: Na, K-ATPase

Author

Grell, E., Saudan, C., Bugnon, P., Lewitzki, E., Merbach, A. E., and Winter, Roland, editor

Published

2003

2. Steroid profiles of professional soccer players: an international comparative study

Author

Strahm, E, Sottas, P-E, Schweizer, C, Saugy, M, Dvorak, J, and Saudan, C

Published

2009

3. Detection of testosterone administration based on the carbon isotope ratio profiling of endogenous steroids: international reference populations of professional soccer players

Author

Strahm, E, Emery, C, Saugy, M, Dvorak, J, and Saudan, C

Published

2009

4. Steroid profiles and professional soccer players: an international comparative study

Author

Strahm, E., Sottas, P.-E., Schweizer, C., Saugy, M., Dvorak, J., and Saudan, C.

Subjects

Soccer players -- Drug use, Soccer players -- Research, Drugs and athletes -- Research, Testosterone -- Analysis, Gas chromatography -- Usage, Mass spectrometry -- Usage, Health, Sports and fitness

Published

2009

5. Human growth hormone doping in sport

Author

Saugy, M, Robinson, N, Saudan, C, Baume, N, Avois, L, and Mangin, P

Published

2006

6. Testosterone and doping control

Author

Saudan, C, Baume, N, Robinson, N, Avois, L, Mangin, P, and Saugy, M

Published

2006

7. Cannabis and sport

Author

Saugy, M, Avois, L, Saudan, C, Robinson, N, Giroud, C, Mangin, P, and Dvorak, J

Published

2006

8. Erythropoietin and blood doping

Author

Robinson, N, Giraud, S, Saudan, C, Baume, N, Avois, L, Mangin, P, and Saugy, M

Published

2006

9. Central nervous system stimulants and sport practice

Author

Avois, L, Robinson, N, Saudan, C, Baume, N, Mangin, P, and Saugy, M

Published

2006

10. Simple and dendritic cyclam derivative. Photophysical properties, effect of protonation and Zn++ coordination, preliminary screening as inhibitors of tumor cell growth

Author

SAUDAN C, VICINELLI V, GORKA M, LEE S. K, VOGTLE F, CERONI, PAOLA, BALZANI, VINCENZO, ORLANDI, MARINA, BARTOLINI, GIOVANNA, TAVOLARI, SIMONA, ROCCHI, PAOLA, FERRERI, ANNA MARIA, SAUDAN C, CERONI P, VICINELLI V, BALZANI V, GORKA M, LEE S-K, VOGTLE F, ORLANDI M, BARTOLINI G., TAVOLARI S, ROCCHI P, and FERRERI AM

Published

2004

11. Analytical science: development of an IRMS technology for tracing gamma-hydroxybutyric acid (GHB)

Author

Pazos, D., Marclay, F., Saudan, C., Delémont, O., and Esseiva, P.

Published

2010

12. Development of an IRMS technology for tracing gamma-hydroxybutyric acid (GHB)

Author

Pazos, D., primary, Marclay, F., additional, Saudan, C., additional, Delémont, O., additional, and Esseiva, P., additional

Published

2010

13. Short-term stability of testosterone and epitestosterone conjugates in urine samples: Quantification by liquid chromatography–linear ion trap mass spectrometry

Author

SAUDAN, C, primary, ENTENZA, J, additional, BAUME, N, additional, MANGIN, P, additional, and SAUGY, M, additional

Published

2006

14. Bayesian detection of abnormal values in longitudinal biomarkers with an application to T/E ratio

Author

Sottas, P.-E., primary, Baume, N., additional, Saudan, C., additional, Schweizer, C., additional, Kamber, M., additional, and Saugy, M., additional

Published

2006

15. Urinary marker of oral pregnenolone administration

Author

SAUDAN, C, primary, DESMARCHELIER, A, additional, SOTTAS, P, additional, MANGIN, P, additional, and SAUGY, M, additional

Published

2005

16. Urinary analysis of 16(5α)-androsten-3α-ol by gas chromatography/combustion/isotope ratio mass spectrometry: implications in anti-doping analysis

Author

SAUDAN, C, primary, BAUME, N, additional, MANGIN, P, additional, and SAUGY, M, additional

Published

2004

17. Urinary Analysis of Four Testosterone Metabolites and Pregnanediol by Gas Chromatography-Combustion-Isotope Ratio Mass Spectrometry after Oral Administrations of Testosterone

Author

Maitre, A., primary, Saudan, C., additional, Mangin, P., additional, and Saugy, M., additional

Published

2004

18. Source inference of exogenous gamma-hydroxybutyric acid (GHB) administered to humans by means of carbon isotopic ratio analysis: novel perspectives regarding forensic investigation and intelligence issues.

Author

Marclay F, Saudan C, Vienne J, Tafti M, and Saugy M

Subjects

Adult, Gas Chromatography-Mass Spectrometry, Humans, Hydroxybutyrates administration & dosage, Hydroxybutyrates pharmacokinetics, Illicit Drugs, Male, Substance Abuse Detection methods, Carbon Isotopes analysis, Forensic Medicine methods, Hydroxybutyrates urine

Abstract

γ-Hydroxybutyric acid (GHB) is an endogenous short-chain fatty acid popular as a recreational drug due to sedative and euphoric effects, but also often implicated in drug-facilitated sexual assaults owing to disinhibition and amnesic properties. Whilst discrimination between endogenous and exogenous GHB as required in intoxication cases may be achieved by the determination of the carbon isotope content, such information has not yet been exploited to answer source inference questions of forensic investigation and intelligence interests. However, potential isotopic fractionation effects occurring through the whole metabolism of GHB may be a major concern in this regard. Thus, urine specimens from six healthy male volunteers who ingested prescription GHB sodium salt, marketed as Xyrem(®), were analysed by means of gas chromatography/combustion/isotope ratio mass spectrometry to assess this particular topic. A very narrow range of δ(13)C values, spreading from -24.81‰ to -25.06‰, was observed, whilst mean δ(13)C value of Xyrem(®) corresponded to -24.99‰. Since urine samples and prescription drug could not be distinguished by means of statistical analysis, carbon isotopic effects and subsequent influence on δ(13)C values through GHB metabolism as a whole could be ruled out. Thus, a link between GHB as a raw matrix and found in a biological fluid may be established, bringing relevant information regarding source inference evaluation. Therefore, this study supports a diversified scope of exploitation for stable isotopes characterized in biological matrices from investigations on intoxication cases to drug intelligence programmes.

Published

2011

19. Potential of IRMS technology for tracing gamma-butyrolactone (GBL).

Author

Marclay F, Pazos D, Delémont O, Esseiva P, and Saudan C

Abstract

Popularity of gamma-hydroxybutyric acid (GHB) is fairly stable among drug users, while the consumption of its chemical precursor, gamma-butyrolactone (GBL), is a growing phenomenon. Although conventional analytical methods allow to detect this substance in various matrices, linking a trace and a source is still a difficult challenge. However, as several synthesis pathways and chemical precursors exist for the production of GBL, its carbon isotopic signature may vary extensively. For that purpose, a method has been developed to determine the carbon isotopes content of GBL by means of gas chromatography/combustion/isotope ratio mass spectrometry (GC/C/IRMS). The delta(13)C-values of 19 bulk samples purchased worldwide were in the range from -23.1 to -45.8 per thousand (SD<0.3 per thousand). Furthermore, testing on the purification of GBL by distillation has not been found to be consistent with such a large range of delta(13)C-values, which are likely to result from the isotopic composition of the organic precursors used to produce GBL together with the kinetic isotope effect associated with the synthesis routes. Finally, inter- and intra-variability measurements of the delta(13)C-values demonstrated the high potential of IRMS for discriminating between seizures of GBL and for source determination.

Published

2010

20. Endogenous steroid profiling in the athlete biological passport.

Author

Sottas PE, Saugy M, and Saudan C

Subjects

Age Factors, Anabolic Agents administration & dosage, Androgens administration & dosage, Androstane-3,17-diol analysis, Bayes Theorem, Biomarkers analysis, Dehydroepiandrosterone analysis, Epitestosterone analysis, Etiocholanolone analysis, Female, Genetic Variation, Humans, Male, Physical Endurance drug effects, Physical Endurance physiology, Reference Values, Sex Factors, Testosterone analysis, Testosterone physiology, Anabolic Agents analysis, Androgens analysis, Athletes, Doping in Sports prevention & control

Abstract

The Athlete Biological Passport (ABP) is an individual electronic document that collects data regarding a specific athlete that is useful in differentiating between natural physiologic variations of selected biomarkers and deviations caused by artificial manipulations. A subsidiary of the endocrine module of the ABP, that which here is called Athlete Steroidal Passport (ASP), collects data on markers of an altered metabolism of endogenous steroidal hormones measured in urine samples. The ASP aims to identify not only doping with anabolic-androgenic steroids, but also most indirect steroid doping strategies such as doping with estrogen receptor antagonists and aromatase inhibitors. Development of specific markers of steroid doping, use of the athlete's previous measurements to define individual limits, with the athlete becoming his or her own reference, the inclusion of heterogeneous factors such as the UDPglucuronosyltransferase B17 genotype of the athlete, the knowledge of potentially confounding effects such as heavy alcohol consumption, the development of an external quality control system to control analytical uncertainty, and finally the use of Bayesian inferential methods to evaluate the value of indirect evidence have made the ASP a valuable alternative to deter steroid doping in elite sports. The ASP can be used to target athletes for gas chromatography/combustion/ isotope ratio mass spectrometry (GC/C/IRMS) testing, to withdraw temporarily the athlete from competing when an abnormality has been detected, and ultimately to lead to an antidoping infraction if that abnormality cannot be explained by a medical condition. Although the ASP has been developed primarily to ensure fairness in elite sports, its application in endocrinology for clinical purposes is straightforward in an evidence-based medicine paradigm., (Copyright 2010 Elsevier Inc. All rights reserved.)

Published

2010

21. Detection in urine of 4-methyl-2-hexaneamine, a doping agent.

Author

Perrenoud L, Saugy M, and Saudan C

Subjects

Amines chemistry, Amines pharmacokinetics, Chromatography, Liquid methods, Doping in Sports, Gas Chromatography-Mass Spectrometry methods, Humans, Reproducibility of Results, Tandem Mass Spectrometry methods, Amines urine

Abstract

Stimulants are banned in-competition for all categories of sports by the World Anti-Doping Agency. A simple liquid chromatography-tandem mass spectrometry (LC-MS/MS) assay employing electrospray ionisation in positive mode was developed in that work for the quantification in urine specimens of 4-methyl-2-hexaneamine, a primary amine exhibiting sympathomimetic properties. Following a simple pretreatment procedure, the analyte was separated using a gradient mobile phase on reverse phase C8 column. Selected reaction monitoring m/z 116.2-->57.3 was specific for detection of 4-methyl-2-hexaneamine and the assay exhibited a linear dynamic range of 50-700 ng/mL. The validated method has been successfully applied to analyze the target compound in food supplements as well as in urine specimens. The administered drug (40 mg) was detected at the level of 350 ng/mL in the urine up to 4 days.

Published

2009

22. The fight against doping: back on track with blood.

Author

Saugy M, Robinson N, and Saudan C

Subjects

Central Nervous System Stimulants urine, Doping in Sports trends, Genomics trends, Humans, Illicit Drugs urine, Metabolomics trends, Prevalence, Program Development methods, Proteomics trends, Central Nervous System Stimulants blood, Data Collection methods, Doping in Sports methods, Illicit Drugs blood

Published

2009

23. Validation and performance comparison of two carbon isotope ratio methods to control the misuse of androgens in humans.

Author

Saudan C, Emery C, Marclay F, Strahm E, Mangin P, and Saugy M

Subjects

Chromatography, Gas methods, Chromatography, High Pressure Liquid methods, Doping in Sports, Mass Spectrometry methods, Androgens urine, Carbon Isotopes analysis, Substance Abuse Detection methods, Testosterone urine

Abstract

Carbon isotope ratio of androgens in urine specimens is routinely determined to exclude an abuse of testosterone or testosterone prohormones by athletes. Increasing application of gas chromatography/combustion/isotope ratio mass spectrometry (GC/C/IRMS) in the last years for target and systematic investigations on samples has resulted in the demand for rapid sample throughput as well as high selectivity in the extraction process particularly in the case of conspicuous samples. For that purpose, we present herein the complimentary use of an SPE-based assay and an HPLC fractionation method as a two-stage strategy for the isolation of testosterone metabolites and endogenous reference compounds prior to GC/C/IRMS analyses. Assays validation demonstrated acceptable performance in terms of intermediate precision (range: 0.1-0.4 per thousand) and Bland-Altman analyses revealed no significant bias (0.2 per thousand). For further validation of this two-stage analyses strategy, all the specimens (n=124) collected during a major sport event were processed.

Published

2009

24. Profiling of 19-norandrosterone sulfate and glucuronide in human urine: implications in athlete's drug testing.

Author

Strahm E, Baume N, Mangin P, Saugy M, Ayotte C, and Saudan C

Subjects

Adult, Chromatography, Liquid, Corticosterone urine, Gas Chromatography-Mass Spectrometry, Humans, Male, Tandem Mass Spectrometry, Young Adult, Corticosterone analogs & derivatives, Doping in Sports, Estranes urine, Substance Abuse Detection methods

Abstract

19-Norandrosterone (19-NA) as its glucuronide derivative is the target metabolite in anti-doping testing to reveal an abuse of nandrolone or nandrolone prohormone. To provide further evidence of a doping with these steroids, the sulfoconjugate form of 19-norandrosterone in human urine might be monitored as well. In the present study, the profiling of sulfate and glucuronide derivatives of 19-norandrosterone together with 19-noretiocholanolone (19-NE) were assessed in the spot urines of 8 male subjects, collected after administration of 19-nor-4-androstenedione (100mg). An LC/MS/MS assay was employed for the direct quantification of sulfoconjugates, whereas a standard GC/MS method was applied for the assessment of glucuroconjugates in urine specimens. Although the 19-NA glucuronide derivative was always the most prominent at the excretion peak, inter-individual variability of the excretion patterns was observed for both conjugate forms of 19-NA and 19-NE. The ratio between the glucuro- and sulfoconjugate derivatives of 19-NA and 19-NE could not discriminate the endogenous versus the exogenous origin of the parent compound. However, after ingestion of 100mg 19-nor-4-androstenedione, it was observed in the urine specimens that the sulfate conjugates of 19-NA was detectable over a longer period of time with respect to the other metabolites. These findings indicate that more interest shall be given to this type of conjugation to deter a potential doping with norsteroids.

Published

2009

25. Doping: a paradigm shift has taken place in testing.

Author

Sottas PE, Saudan C, and Saugy M

Subjects

Humans, Male, Sports standards, Doping in Sports prevention & control, Forensic Sciences methods, Forensic Sciences standards, Substance Abuse Detection methods, Substance Abuse Detection standards

Published

2008

26. Isolation and quantification by high-performance liquid chromatography-ion-trap mass spectrometry of androgen sulfoconjugates in human urine.

Author

Strahm E, Kohler I, Rudaz S, Martel S, Carrupt PA, Veuthey JL, Saugy M, and Saudan C

Subjects

Androgens analysis, Androgens isolation & purification, Androsterone analysis, Androsterone isolation & purification, Androsterone urine, Dehydroepiandrosterone analysis, Dehydroepiandrosterone isolation & purification, Dehydroepiandrosterone urine, Epitestosterone analysis, Epitestosterone isolation & purification, Epitestosterone urine, Etiocholanolone analysis, Etiocholanolone isolation & purification, Etiocholanolone urine, Humans, Reproducibility of Results, Solid Phase Extraction, Testosterone analysis, Testosterone isolation & purification, Testosterone urine, Androgens urine, Chromatography, High Pressure Liquid methods, Mass Spectrometry methods

Abstract

Together with steroid glucuronides, sulfoconjugates may be used as markers of steroid administration as well as endogenous steroid production. A fast and sensitive analytical procedure has been developed for the simultaneous separation, determination and quantification of sulfate and glucuronide derivatives of testosterone (T), epitestosterone (E), androsterone (A), etiocholanolone (Etio) and dehydroepiandrosterone (DHEA) in human urine. First, a weak anion-exchange solid-phase extraction support (SPE Oasis WAX) was used for complete and rapid separation of sulfates and glucuronides in two extracts after loading of urine sample (2 mL). Then sulfates were analyzed directly by high-performance liquid chromatography-ion-trap mass spectrometry (LC-MS/MS) with electrospray ionization in negative mode. Chromatographic separation of the targeted sulfoconjugates was achieved using a Waters XBridge C18 column (150 mm x 4.6 mm I.D., 5 microm) with gradient elution. Assay validation demonstrated good performance for instance for T sulfate (TS) and E sulfate (ES) in terms of trueness (89-107%), repeatability (3.4-22%) and intermediate precision (5.8-22%) over the range of 2-200 ng/mL (corresponding to 1.5-147 ng/mL as free steroids). Results obtained on biological samples demonstrated the suitability of this analytical strategy for direct measurement of androgen sulfoconjugates and glucuroconjugates in human urine.

Published

2008

27. Short term impact of Tribulus terrestris intake on doping control analysis of endogenous steroids.

Author

Saudan C, Baume N, Emery C, Strahm E, and Saugy M

Subjects

Adult, Androstenols urine, Androsterone urine, Etiocholanolone urine, Female, Humans, Luteinizing Hormone urine, Mass Spectrometry methods, Radioimmunoassay, Dehydroepiandrosterone urine, Dietary Supplements, Doping in Sports, Tribulus

Abstract

Tribulus terrestris is a nutritional supplement highly debated regarding its physiological and actual effects on the organism. The main claimed effect is an increase of testosterone anabolic and androgenic action through the activation of endogenous testosterone production. Even if this biological pathway is not entirely proven, T. terrestris is regularly used by athletes. Recently, the analysis of two female urine samples by GC/C/IRMS (gas chromatography/combustion/isotope-ratio-mass-spectrometry) conclusively revealed the administration of exogenous testosterone or its precursors, even if the testosterone glucuronide/epitestosterone glucuronide (T/E) ratio and steroid marker concentrations were below the cut-off values defined by World Anti-Doping Agency (WADA). To argue against this adverse analytical finding, the athletes recognized having used T. terrestris in their diet. In order to test this hypothesis, two female volunteers ingested 500 mg of T. terrestris, three times a day and for two consecutive days. All spot urines were collected during 48 h after the first intake. The (13)C/(12)C ratio of ketosteroids was determined by GC/C/IRMS, the T/E ratio and DHEA concentrations were measured by GC/MS and LH concentrations by radioimmunoassay. None of these parameters revealed a significant variation or increased above the WADA cut-off limits. Hence, the short-term treatment with T. terrestris showed no impact on the endogenous testosterone metabolism of the two subjects.

Published

2008

28. Profiling of 19-norsteroid sulfoconjugates in human urine by liquid chromatography mass spectrometry.

Author

Strahm E, Rudaz S, Veuthey JL, Saugy M, and Saudan C

Subjects

Humans, Reproducibility of Results, Sensitivity and Specificity, Chromatography, Liquid methods, Spectrometry, Mass, Electrospray Ionization methods, Steroids urine, Tandem Mass Spectrometry methods

Abstract

19-Nortestosterone (nandrolone) major metabolites in human urine are excreted as sulfoconjugated and glucuroconjugated forms. A sensitive and selective liquid chromatography/tandem mass spectrometry (LC/MS/MS) method in negative ESI mode was developed for direct quantification of 19-norandrosterone sulfate (19-NAS) and 19-noretiocholanolone sulfate (19-NES). For both sulfoconjugates, the [M-H](-) ion at m/z 355 and the fragment ion at m/z 97 were used as the precursor and product ions, respectively. The purification method involved a complete and rapid separation of sulfates and glucuronides in two extracts after loading the sample on a weak anion exchange solid phase extraction support (SPE Oasis WAX). Then, sulfates were separated by LC (Uptisphere ODB, 150 mm x 3.0 mm, 5 microm) and analyzed on a linear trap and a triple quadrupole mass spectrometer. The lower limit of detection (LLOD) and lowest limit of quantification (LLOQ) were of 100 pg mL(-1) and 1 ng mL(-1), respectively. Assay validation demonstrated good performances in terms of trueness (92.0-104.9%), repeatability (0.6-7.2%) and intermediate precision (1.3-10.8%) over the range of 1-2500 ng mL(-1). Finally, 19-NAS and 19-NES in urine samples collected after intake of 19-norandrostenedione (nandrolone precursor) were quantified. This assay may be easily implemented to separate glucuronide and sulfate steroids from urine specimens prior to quantification by LC/MS/MS.

Published

2008

29. From population- to subject-based limits of T/E ratio to detect testosterone abuse in elite sports.

Author

Sottas PE, Saudan C, Schweizer C, Baume N, Mangin P, and Saugy M

Subjects

Bayes Theorem, Biomarkers urine, Clinical Trials as Topic, False Positive Reactions, Female, Forensic Toxicology, Gas Chromatography-Mass Spectrometry, Glucuronosyltransferase genetics, Humans, Male, Minor Histocompatibility Antigens, Polymorphism, Genetic, Sensitivity and Specificity, Substance Abuse Detection methods, Testosterone administration & dosage, Testosterone analogs & derivatives, Testosterone Congeners administration & dosage, Doping in Sports, Epitestosterone urine, Testosterone urine

Abstract

In elite sports, indirect testing of testosterone abuse is mainly based on the testosterone over epitestosterone (T/E) ratio. Since this marker is characterized by a small ratio of intra- to inter-individual variation, it is surprising that current anti-doping strategy uses a screening test based on a population-based limit. From a database of more than 15,000 steroid profiles obtained from routine controls, the collection of steroids profiles of 11 elite athletes followed during 2 years, and a longitudinal study involving 17 amateur athletes, 8 of which were orally administrated testosterone undecanoate pills, we selected 12 case studies to represent the possible scenarios to which the anti-doping laboratories are confronted. Various detection strategies at the disposal of the laboratories are employed and discussed, including isotope ratio mass spectrometry (IRMS) analysis and a Bayesian interpretation of the T/E-time profile. The weak sensitivity versus specificity relation of a population-based limit for the T/E ratio is outlined. As a result, we propose a Bayesian screening test whose T/E threshold progressively evolves from a population basis to a subject basis as the number of individual test results increases. We found that this screening test heightens drastically the capacity to detect testosterone abuse, at no additional financial and administrative expenses for anti-doping authorities.

Published

2008

30. Direct detection and quantification of 19-norandrosterone sulfate in human urine by liquid chromatography-linear ion trap mass spectrometry.

Author

Strahm E, Saudan C, Sottas PE, Mangin P, and Saugy M

Subjects

Humans, Reference Standards, Reproducibility of Results, Sensitivity and Specificity, Chromatography, Liquid methods, Estranes urine, Spectrometry, Mass, Electrospray Ionization methods, Tandem Mass Spectrometry methods

Abstract

19-Norandrosterone sulfate (19-NAS) is the sulfoconjugated form of 19-norandrosterone (19-NA), the major metabolite of the steroid nandrolone. A sensitive and accurate liquid chromatography/tandem mass spectrometry (LC-MS/MS) assay was developed for the direct measurement of 19-NAS in human urine samples. The method involved a quaternary amine SPE protocol and subsequently injection of the extract onto an analytical column (Uptisphere ODB, 150 mm x 3.0 mm, 5 microm) for chromatographic separation and mass spectrometry detection in negative electrospray ionisation mode. The sulfoconjugate of 19-NA was identified in urine by comparison of mass spectra and retention time with a reference substance. The limit of detection (LOD) and lowest limit of quantification (LLOQ) of 19-NAS were of 40 pg/mL and 200 pg/mL, respectively. For a nominal concentration of 2 ng/mL, recovery (94%), intra-day precision (2.7%), intra-assay precision (6.6%) and inter-assay precision (14.3%) were determined. Finally, this analytical method was applied for quantifying the concentration of 19-NAS in doping samples, using calibration curves (0.2-20 ng/mL) and the standard-addition method. The results show the feasibility of applying this LC-MS/MS assay as a complementary tool to detect misuse of nandrolone or nandrolone precursors.

Published

2007

31. Bayesian detection of abnormal values in longitudinal biomarkers with an application to T/E ratio.

Author

Sottas PE, Baume N, Saudan C, Schweizer C, Kamber M, and Saugy M

Subjects

Biomarkers analysis, Biomarkers urine, Doping in Sports, Humans, Male, Sensitivity and Specificity, Bayes Theorem, Data Interpretation, Statistical, Epitestosterone urine, Longitudinal Studies, Models, Statistical, Testosterone urine

Abstract

We developed a test that compares sequential measurements of a biomarker against previous readings performed on the same individual. A probability mass function expresses prior information on interindividual variations of intraindividual parameters. Then, the model progressively integrates new readings to more accurately quantify the characteristics of the individual. This Bayesian framework generalizes the two main approaches currently used in forensic toxicology for the detection of abnormal values of a biomarker. The specificity is independent of the number n of previous test results, with a model that gradually evolves from population-derived limits when n = 0 to individual-based cutoff thresholds when n is large. We applied this model to detect abnormal values in an athlete's steroid profile characterized by the testosterone over epitestosterone (T/E) marker. A cross-validation procedure was used for the estimation of prior densities as well as model validation. The heightened sensitivity/specificity relation obtained on a large data set shows that longitudinal monitoring of an athlete's steroid profile may be used efficiently to detect the abuse of testosterone and its precursors in sports. Mild assumptions make the model interesting for other areas of forensic toxicology.

Published

2007

32. Performance characteristics of two immunoassays for the measurement of urinary luteinizing hormone.

Author

Robinson N, Saudan C, Sottas PE, Mangin P, and Saugy M

Subjects

Adult, Cross Reactions, Female, Freezing, Humans, Immunoassay, Immunoenzyme Techniques, Male, Reproducibility of Results, Specimen Handling, Sports, Doping in Sports, Luteinizing Hormone urine

Abstract

Urine luteinizing hormone (LH) concentration is routinely measured in all anti-doping laboratories to exclude recombinant LH abuse and to test any potential alteration of the hypophyseal-gonadal axis. Before establishing proper reference values among professional top level athletes, an extended validation of two commercial immunoassays for LH measurements was performed. Elecsys 1010 and Access are two automated immunoanalyzers for central laboratories. The limit of detection, the limit of quantification, intra-laboratory, inter-technique correlation, precision, accuracy were determined. Furthermore, reference urinary LH distribution values for male and female top level athletes were determined. Stability studies of LH in urine following freezing and thawing cycles (n=3) as well as storage conditions at room temperature, 4 degrees C and -20 degrees C were performed. Male and female subjects showed important urinary corrected (specific gravity correction) LH distribution differences. Intra-assay precision for the Access analyzer was less than 8.0% whereas inter-assay was close to 11%. Intra and inter-assay precision for the Elecsys 1010 analyzer was slightly better. A good inter-technique correlation was obtained ([Elecsys 1010]=1.0434[Access]+1.146, R=0.953). No urinary LH loss was observed after two freezing and thawing cycles. On the other hand, time and bad storage conditions such as elevated temperature can deteriorate rapidly urinary LH. In conclusion, both analyzers showed acceptable performances and are suitable for screening anti-doping analyses. Each anti-doping laboratory has to settle its own reference distribution values and then determine when to launch a confirmation procedure. This takes place then depending on the positivity criteria the anti-doping laboratory has established and validated. This study also clearly showed that the time delay between the urine collection and the analysis should be reduced as much as possible and urine samples should be transported in optimal conditions (low temperature and quickly) to decrease urinary LH deterioration.

Published

2007

33. Carbon isotopic ratio analysis by gas chromatography/combustion/isotope ratio mass spectrometry for the detection of gamma-hydroxybutyric acid (GHB) administration to humans.

Author

Saudan C, Augsburger M, Mangin P, and Saugy M

Subjects

Carbon Isotopes analysis, Forensic Medicine methods, Humans, Hydroxybutyrates pharmacokinetics, Reproducibility of Results, Gas Chromatography-Mass Spectrometry methods, Hydroxybutyrates urine, Substance Abuse Detection methods

Abstract

Since GHB (gamma-hydroxybutyric acid) is naturally produced in the human body, clinical and forensic toxicologists must be able to discriminate between endogenous levels and a concentration resulting from exposure. To suggest an alternative to the use of interpretative concentration cut-offs, the detection of exogenous GHB in urine specimens was investigated by means of gas chromatography/combustion/isotope ratio mass spectrometry (GC/C/IRMS). GHB was isolated from urinary matrix by successive purification on Oasis MCX and Bond Elute SAX solid-phase extraction (SPE) cartridges prior to high-performance liquid chromatography (HPLC) fractioning using an Atlantis dC18 column eluted with a mixture of formic acid and methanol. Subsequent intramolecular esterification of GHB leading to the formation of gamma-butyrolactone (GBL) was carried out to avoid introduction of additional carbon atoms for carbon isotopic ratio analysis. A precision of 0.3 per thousand was determined using this IRMS method for samples at GHB concentrations of 10 mg/L. The (13)C/(12)C ratios of GHB in samples of subjects exposed to the drug ranged from -32.1 to -42.1 per thousand, whereas the results obtained for samples containing GHB of endogenous origin at concentration levels less than 10 mg/L were in the range -23.5 to -27.0 per thousand. Therefore, these preliminary results show that a possible discrimination between endogenous and exogenous GHB can be made using carbon isotopic ratio analyses., (Copyright (c) 2007 John Wiley & Sons, Ltd.)

Published

2007

34. Elevated and similar urinary testosterone/epitestosterone ratio in all samples of a competition testing: suspicion of a manipulation.

Author

Robinson N, Castella V, Saudan C, Sottas PE, Schweizer C, Dimo-Simonin N, Mangin P, and Saugy M

Subjects

DNA Fingerprinting, Gas Chromatography-Mass Spectrometry, Humans, Substance Abuse Detection, Bicycling, Doping in Sports, Epitestosterone urine, Specimen Handling standards, Testosterone urine

Abstract

The case of seven urine samples collected for anti-doping purposes during a cycling stage race with moderately elevated testosterone and epitestosterone ratio (T/E) is reported. The very low probability of having all seven urine samples with such similar elevated T/E ratio (from 3.2 to 4.7) was very suspicious. Different pattern classification tools were tested to categorize the most similar steroid profiles, but none of the models enabled a clear classification of the different urine samples. Subsequently, genetic profiling of all urine samples was performed and demonstrated that three of the seven samples were collected from the same cyclist. Finally, the International Federation confirmed DNA profiling results. This suggests that urinary steroid data using several methodologies are not appropriate for identification purposes and to an extent not unique to individuals.

Published

2006

35. Use of isotope ratio mass spectrometry to detect doping with oral testosterone undecanoate: inter-individual variability of 13C/12C ratio.

Author

Baume N, Saudan C, Desmarchelier A, Strahm E, Sottas PE, Bagutti C, Cauderay M, Schumacher YO, Mangin P, and Saugy M

Subjects

Administration, Oral, Adult, Carbon Isotopes, Gas Chromatography-Mass Spectrometry methods, Humans, Male, Reference Values, Testosterone administration & dosage, Testosterone metabolism, Testosterone urine, Time Factors, Doping in Sports, Genetic Variation, Substance Abuse Detection methods, Testosterone analogs & derivatives

Abstract

The metabolic effect of multiple oral testosterone undecanoate (TU) doses over 4 weeks was assessed in seven voluntary men. The protocol was designed to detect accumulation of the substance by choosing the appropriate spot urines collections time and to study the urinary clearance of the substance after weeks of treatment. Urines were analysed by a new GC/C/isotope ratio mass spectrometry (IRMS) method to establish the delta(13)C-values of testosterone metabolites (androsterone and etiocholanolone) together with an endogenous reference compound (16(5alpha)-androsten-3alpha-ol). The significant differences in inter-individual metabolism following TU intake was illustrated by large variations in delta(13)C-values of both T metabolites (maximum Deltadelta(13)C-values = 5.5 per thousand), as well as by very stable longitudinal T/E profiles and carbon isotopic ratios in the first hours following administration. According to T/E ratios and delta(13)C-values, the washout period after 80 mg TU intake was less than 48 h for all subjects and no accumulation phenomenon was observed upon chronic oral administration.

Published

2006

36. Longitudinal profiling of urinary steroids by gas chromatography/combustion/isotope ratio mass spectrometry: diet change may result in carbon isotopic variations.

Author

Saudan C, Kamber M, Barbati G, Robinson N, Desmarchelier A, Mangin P, and Saugy M

Subjects

Adult, Carbon Isotopes analysis, Doping in Sports, Epitestosterone urine, Humans, Kenya, Longitudinal Studies, Male, Running physiology, South Africa, Switzerland, Testosterone urine, Chromatography, Gas methods, Diet, Mass Spectrometry methods, Steroids urine

Abstract

Longitudinal profiling of urinary steroids was investigated by using a gas chromatography/combustion/isotope ratio mass spectrometry (GC/C/IRMS) method. The carbon isotope ratio of three urinary testosterone (T) metabolites: androsterone, etiocholanolone, 5beta-androstane-3alpha,17beta-diol (5beta-androstanediol) together with 16(5alpha)-androsten-3alpha-ol (androstenol) and 5beta-pregnane-3alpha,20alpha-diol (5beta-pregnanediol) were measured in urine samples collected from three top-level athletes over 2 years. Throughout the study, the subjects were living in Switzerland and were residing every year for a month or two in an African country. (13)C-enrichment larger than 2.5 per thousand was observed for one subject after a 2-month stay in Africa. Our findings reveal that (13)C-enrichment caused by a diet change might be reduced if the stay in Africa was shorter or if the urine sample was not collected within the days after return to Switzerland. The steroids of interest in each sample did not show significant isotopic fractionation that could lead to false positive results in anti-doping testing. In contrast to the results obtained with the carbon isotopic ratio, profiling of urinary testosterone/epitestosterone (T/E) ratios was found to be unaffected by a diet change.

Published

2006

37. Detection of exogenous GHB in blood by gas chromatography-combustion-isotope ratio mass spectrometry: implications in postmortem toxicology.

Author

Saudan C, Augsburger M, Kintz P, Saugy M, and Mangin P

Subjects

Carbon Isotopes, Humans, Forensic Medicine methods, Gas Chromatography-Mass Spectrometry methods, Sodium Oxybate blood, Substance Abuse Detection methods

Abstract

Because GHB (gamma-hydroxybutyrate) is present in both blood and urine of the general population, toxicologists must be able to discriminate between endogenous levels and a concentration resulting from exposure. In this paper, we propose a procedure for the detection of exogenous GHB in blood by gas chromatography-combustion-isotope ratio mass spectrometry (GC-C-IRMS). Following liquid-liquid and solid-phase extractions, GHB is derivatized to GHB di-TMS before analysis by GC-C-IRMS. Significant differences in the carbon isotopic ratio (delta(13)C-values > 13.5 per thousand) were found between endogenous and synthetic GHB. Indeed, for postmortem blood samples with different GHB concentrations (range: 13.8-86.3 mg/L), we have obtained GHB delta(13)C-values ranging from -20.6 to -24.7 per thousand, whereas delta(13)C-values for the GHB from police seizure were in the range -38.2 to -50.2 per thousand. In contrast to the use of cut-off concentrations for positive postmortem blood GHB concentrations, this method should provide an unambiguous indication of the drug origin.

Published

2005

38. Proton-driven self-assembled systems based on cyclam-cored dendrimers and [Ru(bpy)(CN)4]2-.

Author

Bergamini G, Saudan C, Ceroni P, Maestri M, Balzani V, Gorka M, Lee SK, van Heyst J, and Vögtle F

Abstract

1,4,8,11-tetraazacyclotetradecane (cyclam), which is one of the most extensively investigated ligands in coordination chemistry, in its protonated forms, can play the role of host toward cyanide metal complexes. We have investigated the acid-driven adducts formed in acetonitrile-dichloromethane (1:1 v/v) solution by [Ru(bpy)(CN)4](2-) with 1,4,8,11-tetrakis(naphthylmethyl)cyclam (1) and a dendrimer consisting of a cyclam core appended with 12 dimethoxybenzene and 16 naphthyl units (2). [Ru(bpy)(CN)4](2-), 1, and 2 exhibit characteristic absorption and emission bands, in distinct spectral regions, that are strongly affected by addition of acid. When a solution containing equimolar amounts of [Ru(bpy)(CN)4](2-) and 1 or 2 is titrated by trifluoroacetic acid, or when [Ru(bpy)(CN)4](2-) is titrated with (1.2H)2+ or (2.2H)2+, [[Ru(bpy)(CN)4](2-).(2H+).1] or [[Ru(bpy)(CN)4](2-).(2H+).2] adducts are formed in which the fluorescence of the naphthyl units is strongly quenched by very efficient energy transfer to the metal complex, as shown by the sensitized luminescence of the latter. The [[Ru(bpy)(CN)4]2-.(2H+).1] and [[Ru(bpy)(CN)4](2-).(2H+).2] adducts can be disrupted (i) by addition of a base (1,4-diazabicyclo[2.2.2]octane), yielding the starting species [Ru(bpy)(CN)4](2-) and 1 or 2, or (ii) by further addition of triflic acid, with formation of (1.2H)2+ or (2.2H)2+ and protonated forms of [Ru(bpy)(CN)4](2-). It is shown that upon stimulation with two chemical inputs (acid and base) both [[Ru(bpy)(CN)4](2-).(2H+).1] and [[Ru(bpy)(CN)4](2-).(2H+).2] exhibit two distinct optical outputs (a naphthalene-based and a Ru(bpy)-based emission) that behave according to an XOR and an XNOR logic, respectively.

Published

2004

39. Cyclam-based dendrimers as ligands for lanthanide ions.

Author

Saudan C, Ceroni P, Vicinelli V, Maestri M, Balzani V, Gorka M, Lee SK, van Heyst J, and Vögtle F

Abstract

We have investigated the complexation of lanthanide ions (Nd3+, Eu3+, Gd3+, Tb3+, Dy3+) with three cyclam-based ligands (cyclam = 1,4,8,11-tetraazacyclotetradecane), namely 1,4,8,11-tetrakis(naphthylmethyl)cyclam (1), and two dendrimers consisting of a cyclam core appended with four dimethoxybenzene and eight naphthyl units (2) and twelve dimethoxybenzene and sixteen naphthyl units (3). In the free ligands the fluorescence of the naphthyl units is strongly quenched by exciplex formation with the cyclam nitrogens. Complexation with the metal ions prevents exciplex formation and revives the intense naphthyl fluorescence. Fluorescence and NMR titration experiments have revealed the formation of complexes with different metal/ligand stoichiometries in the case of 1, 2 and 3. Surprisingly, the large dendrimer 3 gives rise to a stable [M(3)3]3+ species. Energy transfer from the lowest singlet and triplet excited states of the peripheral naphthyl units to the lower lying excited states of Nd3+, Eu3+, Tb3+, Dy3+ coordinated to the cyclam core does not take place.

Published

2004

40. Dendrimers as ligands: an investigation into the stability and kinetics of Zn2+ complexation by dendrimers with 1,4,8,11-tetraazacyclotetradecane (cyclam) cores.

Author

Saudan C, Balzani V, Gorka M, Lee SK, Van Heyst J, Maestri M, Ceroni P, Vicinelli V, and Vögtle F

Abstract

We have investigated the complexation of Zn(2+) with 1,4,8,11-tetrakis(naphthylmethyl) cyclam (1; cyclam=1,4,8,11-tetraazacyclotetradecane) and with two dendrimers consisting of a cyclam core with four dimethoxybenzene and eight naphthyl appendages (2), and twelve dimethoxybenzene and sixteen naphthyl appendages (3). An important, common feature of model compound 1 and dendrimers 2 and 3 is that their potentially fluorescent naphthyl units are quenched by exciplex formation with the cyclam nitrogen atoms. Complexation with Zn(2+), however, prevents exciplex formation and results in the appearance of an intense naphthyl fluorescence signal that can be used for monitoring the complexation process. Luminescence titration, together with competition experiments and (1)H NMR titration, have shown that 1:1 and 1:2 (metal/ligand) complexes are formed in the cases of 2 and 3, whereas model compound 1 gives only a 1:1 complex. We have also investigated the 1:1 complexation kinetics by the stopped-flow technique. In the case of 1, a second-order process (k(1)=44x10(5) M(-1) s(-1)) is followed by two consecutive first-order steps (k(2)=0.53 s(-1) and k(3)=0.10 s(-1)). For 2, a slower second-order process (k(1)=4.9x10(5) M(-1) s(-1)) is followed by a slow first-order step (k(2)=0.40 s(-1)). In the case of 3, only a very slow second-order process was observed (k(1)=1.2x10(5) M(-1) s(-1)). The different metal-ion incorporation rates for model compound 1 and dendrimers 2 and 3 have been discussed in terms of conformational changes of the dendron subunits affecting the chelating properties of the cyclam core. This work reports the first kinetic study on metal-ion coordination by dendrimers with a well-defined coordination site.

Published

2004

41. Dendrimers as ligands. Formation of a 2:1 luminescent complex between a dendrimer with a 1,4,8,11-tetraazacyclotetradecane (cyclam) core and Zn2+.

Author

Saudan C, Balzani V, Gorka M, Lee SK, Maestri M, Vicinelli V, and Vögtle F

Abstract

We have investigated the formation of metal complexes between Zn2+ and two derivatives, 1 and 2, of the well-known 1,4,8,11-tetraazacyclotetradecane (cyclam) ligand. Compound 1 is 1,4,8,11-tetrakis(naphthylmethyl) cyclam, and compound 2 is a dendrimer consisting of a cyclam core with appended 12 dimethoxybenzene and 16 naphthyl units. Compound 1 exhibits an emission band with a maximum around 480 nm, assigned to the formation of exciplexes between amine and excited naphthyl units. Dendrimer 2 exhibits three types of weak emission bands, assigned to naphthyl localized excited states (lambdamax = 337 nm), naphthyl excimers (lambdamax ca. 390 nm), and naphthyl-amine exciplexes (lambdamax = 480 nm). In CH3CN-CH2Cl2 1:1 v/v, titration of ligand 1 with Zn2+ causes the disappearance of the exciplex emission and the appearance of a strong naphthyl localized fluorescence; the titration plot is linear and reaches a plateau for a 1:1 stoichiometry, showing that a highly stable [Zn(1)]2+ complex is formed. In the case of 2, titration with Zn2+ causes the disappearance of the exciplex band, with a concomitant increase in the excimer and naphthyl localized emissions; the titration plot is again linear, but in this case it reaches a plateau for a 2:1 stoichiometric ratio, showing the unexpected formation of a [Zn(2)2]2+ complex. Such an unexpected stoichiometry for the complex of the dendritic ligand has been fully confirmed by 1H NMR titrations. The results obtained show that the dendrimer branches not only do not hinder, but in fact favor coordination of cyclam to Zn2+.

Published

2003

42. Luminescent dendrimers. Recent advances.

Author

Balzani V, Ceroni P, Maestri M, Saudan C, and Vicinelli V

Abstract

Luminescent dendrimers are currently attracting much attention since coupling luminescence and dendrimer research topics can lead to valuable new functions. Indeed, luminescence is a valuable tool to monitor both basic properties and possible applications (sensors, displays, lasers), and dendrimers are macromolecular compounds exhibiting a well-defined chemical structure with the possibility of containing selected chemical units in predetermined sites and of encapsulating ions or neutral molecules in their internal dynamic cavities. In this paper we will review recent advances in this field focusing our attention on their properties in fluid solution related to light harvesting, changing the "color" of light, sensing with signal amplification, quenching and sensitization processes, shielding effects, elucidation of dendritic structures and superstructures, and investigation of dendrimer rotation in solution.

Published

2003

43. Examining reactivity and specificity of cytochrome c peroxidase by using combinatorial mutagenesis.

Author

Wilming M, Iffland A, Tafelmeyer P, Arrivoli C, Saudan C, and Johnsson K

Subjects

Amino Acid Substitution, Cytochrome-c Peroxidase chemistry, Directed Molecular Evolution, Saccharomyces cerevisiae enzymology, Cytochrome-c Peroxidase metabolism, Mutagenesis

Abstract

Combinatorial mutagenesis was used to investigate the role of three key residues in cytochrome c peroxidase (CCP) from Saccharomyces cerevisiae, Arg48, Trp51, and Trp191, in control of the reactivity and selectivity of the heme-containing enzyme. Libraries were prepared by randomization of these residues and were subsequently screened for activity against the phenolic substrate guaiacol. Screening conditions were employed that favor either mutants with high activity or those with both high activity and stability of the reactive enzyme intermediates. The results obtained suggest a dual role for Arg48 of CCP: in addition to stabilizing reactive enzyme intermediates, the distal arginine residue plays a major role in restriction of access to the ferryl oxygen atom by small molecules and thereby controls reactivity and substrate specificity of the peroxidase. At position 51 of CCP, either a phenylalanine or a tryptophan residue is required both for catalytic and structural reasons. In contrast, either polar or positively charged residues are accepted at the position of Trp191, which is located inside the core of the protein. The variability at position 191 can be interpreted as a reflection of the mechanism of cytochrome c peroxidase, which transforms the nonpolar Trp191 into a transient cation radical.

Published

2002

44. Water contributes actively to the rapid crossing of a protein unfolding barrier.

Author

Jacob MH, Saudan C, Holtermann G, Martin A, Perl D, Merbach AE, and Schmid FX

Subjects

Bacillus subtilis chemistry, Guanidines, Kinetics, Pressure, Protein Denaturation, Protein Folding, Recombinant Proteins chemistry, Thermodynamics, Thiocyanates, Urea, Water chemistry, Bacterial Proteins chemistry

Abstract

The cold-shock protein CspB folds rapidly in a N <= => U two-state reaction via a transition state that is about 90% native in its interactions with denaturants and water. This suggested that the energy barrier to unfolding is overcome by processes occurring in the protein itself, rather than in the solvent. Nevertheless, CspB unfolding depends on the solvent viscosity. We determined the activation volumes of unfolding and refolding by pressure-jump and high-pressure stopped-flow techniques in the presence of various denaturants. The results obtained by these methods agree well. The activation volume of unfolding is positive (Delta V(++)(NU)=16(+/-4) ml/mol) and virtually independent of the nature and the concentration of the denaturant. We suggest that in the transition state the protein is expanded and water molecules start to invade the hydrophobic core. They have, however, not yet established favorable interactions to compensate for the loss of intra-protein interactions. The activation volume of refolding is positive as well (Delta V(++)(NU)=53(+/-6) ml/mol) and, above 3 M urea, independent of the concentration of the denaturant. At low concentrations of urea or guanidinium thiocyanate, Delta V(++)(UN) decreases significantly, suggesting that compact unfolded forms become populated under these conditions., ((c) 2002 Elsevier Science Ltd.)

Published

2002

45. A model for sequential threading of alpha-cyclodextrin onto a guest: a complete thermodynamic and kinetic study in water.

Author

Saudan C, Dunand FA, Abou-Hamdan A, Bugnon P, Lye PG, Lincoln SF, and Merbach AE

Subjects

Kinetics, Magnetic Resonance Spectroscopy, Spectrophotometry methods, Thermodynamics, Azo Compounds chemistry, Benzene Derivatives chemistry, Coloring Agents chemistry, Cyclodextrins chemistry, alpha-Cyclodextrins

Abstract

The first variable-temperature and variable-pressure stopped-flow spectrophotometric study of the sequential threading of alpha-cyclodextrin (alpha-CD) onto the guest dye Mordant Orange 10, S, is reported. Complementary (1)H one-dimensional (1D) variable-temperature kinetic studies and two-dimensional (2D) rotating-frame nuclear Overhauser effect spectroscopy (ROESY) and EXSY NMR studies are also reported. In aqueous solution at 298.2 K, the first alpha-CD threads onto S to form a 1:1 complex S.alpha-CD with a forward rate constant k(1,f) = 15 200 +/- 200 M(-1) s(-1) and dethreads with a reverse rate constant k(1,r) = 4.4 +/- 0.3 s(-1). Subsequently, S.alpha-CD isomerizes to S.alpha-CD (k(3,f) = 0.158 +/- 0.006 s(-1), k(3,f) = 0.148 +/- 0.006 s(-1)). This process can be viewed as a thermodynamically controlled molecular shuttle. A second alpha-CD threads onto S.alpha-CD to form a 1:2 complex, S.(alpha-CD)(2), with k(2,f) = 98 +/- 2 M(-1) s(-1) and k(2,r) = 0.032 +/- 0.002 s(-1). A second alpha-CD also threads onto S.alpha-CD to form another 1:2 complex, S.(alpha-CD)(2), characterized by k(4,f) = 9640 +/- 1800 M(-1) s(-1) and k(4,r) = 61 +/- 6 s(-1). Direct interconvertion between S.(alpha-CD)(2) and S.(alpha-CD)(2) was not detected; instead, they interconvert by dethreading the second alpha-CD and through the isomerization equilibrium between S.alpha-CD and S.alpha-CD. The reaction volumes, DeltaV(0), were found to be negative for the first three equilibria and positive for the fourth equilibrium. For the first three forward and reverse reactions, the volumes of activation are substantially more negative, indicating a compression of the transition state in comparison with the ground states. These data were used in conjunction with DeltaH, DeltaH degrees, DeltaS, and DeltaS degrees data to deduce the dominant mechanistic threading processes, which appear to be largely controlled by changes in hydration and van der Waals interactions, and possibly by conformational changes in both S and alpha-CD. The structure of the four complexes were deduced from (1)H 2D ROESY NMR studies.

Published

2001

46. Directed molecular evolution of cytochrome c peroxidase.

Author

Iffland A, Tafelmeyer P, Saudan C, and Johnsson K

Subjects

Alanine chemistry, Alanine genetics, Asparagine chemistry, Asparagine genetics, Aspartic Acid chemistry, Aspartic Acid genetics, Cloning, Molecular methods, Cytochrome-c Peroxidase biosynthesis, Enzyme Activation genetics, Gene Library, Genetic Vectors chemical synthesis, Guaiacol chemistry, Point Mutation, Saccharomyces cerevisiae enzymology, Saccharomyces cerevisiae genetics, Substrate Specificity, Threonine chemistry, Threonine genetics, Tyrosine genetics, Cytochrome-c Peroxidase chemistry, Cytochrome-c Peroxidase genetics, Directed Molecular Evolution methods

Abstract

Cytochrome c peroxidase (CCP) from Saccharomyces cerevisiae was subjected to directed molecular evolution to generate mutants with increased activity against the classical peroxidase substrate guaiacol, thus changing the substrate specificity of CCP from the protein cytochrome c to a small organic molecule. After three rounds of DNA shuffling and screening, mutants were isolated which possessed a 300-fold increased activity against guaiacol and an up to 1000-fold increased specificity for this substrate relative to that for the natural substrate. In all of the selected mutants, the distal arginine (Arg48), which is fully conserved in the superfamily of peroxidases, was mutated to histidine, showing that this mutation plays a key role in the significant increase in activity against phenolic substrates. The results suggest that, in addition to stabilizing the reactive intermediate compound I, the distal arginine plays an important role as a gatekeeper in the active site of CCP, controlling the access to the ferryl oxygen and the distal histidine. Other isolated mutations increase the general reactivity of the peroxidase or increase the intracellular concentration of the active holo form, allowing their selection under the employed screening conditions. The results illustrate the ability of directed molecular evolution technologies to deliver solutions to biochemical problems that would not be readily predicted by rational design.

Published

2000

47. Denaturant-induced movement of the transition state of protein folding revealed by high-pressure stopped-flow measurements.

Author

Pappenberger G, Saudan C, Becker M, Merbach AE, and Kiefhaber T

Subjects

Guanidine, Kinetics, Pressure, Protein Denaturation, Protein Structure, Secondary, Thermodynamics, Peptides chemistry, Protein Folding

Abstract

The small all-beta protein tendamistat folds and unfolds with two-state kinetics. We determined the volume changes associated with the folding process by performing kinetic and equilibrium measurements at variable pressure between 0.1 and 100 MPa (1 to 1, 000 bar). GdmCl-induced equilibrium unfolding transitions reveal that the volume of the native state is increased by 41.4 +/- 2.0 cm(3)/mol relative to the unfolded state. This value is virtually independent of denaturant concentration. The use of a high-pressure stopped-flow instrument enabled us to measure the activation volumes for the refolding (DeltaVo/f) and unfolding reaction (DeltaVo/u) over a broad range of GdmCl concentrations. The volume of the transition state is 60% native-like (DeltaVo/f) = 25.0 +/- 1.2 cm(3)/mol) in the absence of denaturant, indicating partial solvent accessibility of the core residues. The volume of the transition state increases linearly with denaturant concentration and exceeds the volume of the native state above 6 M GdmCl. This result argues for a largely desolvated transition state with packing deficiencies at high denaturant concentrations and shows that the structure of the transition state depends strongly on the experimental conditions.

Published

2000