Rapid monitoring of antibiotics using Raman and surface enhanced Raman spectroscopy

Comparatively few studies have explored the ability of Raman spectroscopy for the quantitative analysis of microbial secondary metabolites in fermentation broths. In this study we investigated the ability of Raman spectroscopy to differentiate between different penicillins and to quantify the level of penicillin in fermentation broths. However, the Raman signal is rather weak, therefore the Raman signal was enhanced using surface enhanced Raman spectroscopy (SERS) employing silver colloids. It was difficult by eye to differentiate between the five different penicillin molecules studied using Raman and SERS spectra, therefore the spectra were analysed by multivariate cluster analysis. Principal components analysis (PCA) clearly showed that SERS rather than the Raman spectra produced reproducible enough spectra to allow for the recovery of each of the different penicillins into their respective five groups. To highlight this further the first five principal components were used to construct a dendrogram using agglomerative clustering, and this again clearly showed that SERS can be used to identify which penicillin molecule was being analysed, despite their molecular similarities. With respect to the quantification of penicillin G it was shown that Raman spectroscopy could be used to quantify the amount of penicillin present in solution when relatively high levels of penicillin were analysed (>50 mM). By contrast, the SERS spectra showed reduced fluorescence, and improved signal to noise ratios from considerably lower concentrations of the antibiotic. This could prove to be advantageous in industry for monitoring low levels of penicillin in the early stages of antibiotic production. In addition, SERS may have advantages for quantifying low levels of high value, low yield, secondary metabolites in microbial processes.     

Realtime Monitoring of Xylitol Fermentation by Micro-Raman Spectroscopy

The fermentation of xylitol is a promising alternative to conventional chemical processes. Micro-Raman spectroscopy was used to monitor the process involving Candida tropicalis, including the medium and yeast cells during xylitol fermentation. The spectra of the fermentation medium showed that the characteristic xylitol peak at 866 cm^?1 was enhanced from 18 h and that the characteristic xylose peak at 901 cm^?1 gradually diminished as the reaction progressed. The characteristic ethanol peak at 880 cm^?1 indicated the production of by-products. Intracellular biological macromolecules, such as nucleic acids, proteins, lipids, and carbohydrates, were identified in the spectra of yeast cells. The intensity of nucleic acids at 783 cm^?1 reached the highest value after 3 h. The xylose band at 901 cm^?1 and the peaks in the carbohydrate region reached a maximum in the logarithmic phase, indicating the carbohydrate metabolism was the most active. The amide I band located at 1658 cm^?1 indicated the major secondary structure of proteins was α-helix; its intensity gradually reduced during the fermentation. The 853 cm^?1 band due to buried tyrosine was predominant at 21 h. In addition, the 1275 cm^?1 band corresponded to the presence of a random coil only at 27 h. These results provided a perspective to understand fermentation and verified the applicability of Raman spectroscopy in xylitol fermentation.     

Surface-enhanced Raman scattering for quantitative detection of ethyl carbamate in alcoholic beverages

Ethyl carbamate, a by-product of fermentation and storage with widespread occurrence in fermented food and alcoholic beverages, is a compound potentially toxic to humans. In this work, a new approach for quantitative detection of ethyl carbamate in alcoholic beverages, based on surface-enhanced Raman scattering (SERS), is reported. Individual silver-coated gold nanoparticle colloids are used as SERS amplifiers, yielding high Raman enhancement of ethyl carbamate in three kinds of alcoholic beverages (vodka, Obstler, and white rum). The characteristic band at 1,003 cm^-1, which is the strongest and best reproducible peak in the SERS spectra, was used for quantitative evaluation of ethyl carbamate. The limit of detection, which corresponds to a signal-to-noise ratio of 3, was 9.0?×?10^-9 M (0.8 μg?·?L^-1), 1.3?×?10^-7 M (11.6 μg?·?L^-1), and 7.8?×?10^-8 M (6.9 μg?·?L^-1), respectively. Surface-enhanced Raman spectroscopy offers great practical potential for the in situ assessment and identification of ethyl carbamate in the alcoholic beverage industry.     

Quantification of moxifloxacin in urine using surface-enhanced Raman spectroscopy (SERS) and multivariate curve resolution on a nanostructured gold surface

A simple procedure is proposed for the determination of the antibiotic moxifloxacin in urine using nanostructured gold as surface-enhanced Raman scattering signal enhancer. The standard addition method in conjunction to multivariate curve resolution-alternating least squares was applied to eliminate the matrix effect and to isolate the spectral contribution of the analyte. Even in the presence of unexpected interferences in the urinary media, it was possible to extract and quantify the analyte response, reaching, in this way, the so-called second-order advantage from first-order data. Moreover, although a saturation phenomenon of the metallic surface was observed, the results of the proposed methodology presented important advantages such as high sensitivity and simpler experimental procedures. The moxifloxacin was determined at levels of 0.70 and 1.50 μg mL^?1 in urine diluted to 1.0 % (corresponding to 70.0 and 150 μg mL^?1 in the original samples) with relative errors of 4.23 and 8.70 %, respectively. The limit of detection (0.085 μg mL^?1) and limit of quantification (0.26 μg mL^?1) values indicated that the quantification can be accomplished in urine up to 24 h after the administration of a single 400-mg dose.     

Rapid determination of illegal additives chrysoidin and malachite green by surface-enhanced Raman scattering with silanized support based substrate

Silanized support based SERS substrate is applied to detect chrysoidin in Sprite at 0.01 mg/L and malachite green in fish pond water at 0.0001 mg/L. The SERS method is sensitive, cost-effective and convenient, which has great potential in detection of illegal additives and harmful substances.     

Development of a Reversed-Phase Liquid Chromatographic Assay for the Quantification of Total Persipeptides in Fermentation Broth

The emergence and prevalence of multi-drug-resistant bacterial strains increase the potential for outbreaks of incurable infections. The discovery of novel antibiotics and pharmacological preparations requires the identification of novel bioactive small molecules. A specific, sensitive, and reliable quantification method using high-performance liquid chromatography (HPLC) with UV detection was developed for the determination of total persipeptides (A and B), which are cyclic pentapeptides found in the fermentation broth of Streptomyces zagrosensis UTMC 1154 that exhibit bioactivity against methicillin-resistant Staphylococcus aureus (MRSA). A simple liquid–liquid extraction (LLE) method using butanol was employed to extract persipeptides from the fermentation broth prior to HPLC analysis. The chromatographic separation of persipeptides and the internal standard, virginiamycin, was achieved with a gradient of acetonitrile and water on a C18 reversed-phase analytical column in a 25-min analytical run utilizing a flow rate of 0.8 mL min⁻¹ and detection at 210 nm. The whole assay was validated, and the method presented a linear response range with a regression coefficient of determination R ² of 0.9996 for the quantification of persipeptides in the concentration range of 3.9–250.0 µg mL⁻¹, as well as extraction recoveries ranging from 54.78 ± 9.83 % to 56.45 ± 16.33 %. The bias and the precision of the proposed method were <10 %. The detection and quantification limits for the persipeptides were 27 and 83 µg L⁻¹, respectively.

     

Online solid-phase extraction–liquid chromatography–electrospray–tandem mass spectrometry determination of multiple classes of antibiotics in environmental and treated waters

An online solid-phase extraction and liquid chromatography in combination with tandem mass spectrometry method was developed for the simultaneous determination of 31 antibiotics in drinking water, surface water and reclaimed waters. The developed methodology requires small sample volume (10 mL), very little sample preparation and total sample run time was 20 min. An Ion Max API heated electrospray ionization source operated in the positive mode with two selected reaction monitoring transitions was used per antibiotic for positive identity and quantification performed by the internal standard approach, to correct for matrix effects and any losses in the online extraction step. Method detection limits were in the range of 1.2–9.7, 2.2–15, 5.5–63 ng/L in drinking water, surface water and reclaimed waters, respectively. The method accuracy in matrix spiked samples ranged from 50–150 % for the studied antibiotics. The applicability of the method was demonstrated using various environmental and reclaimed water matrices. Erythromycin was detected in more than 85 % of the samples in all matrices (28–414, n.d.–199, n.d.–66 ng/L in reclaimed, river and drinking waters respectively). The other frequently detected antibiotics in reclaimed waters were nalidixic acid, clarithromycin, azithromycin, trimethoprim, and sulfamethoxazole.     

Structural and optical properties of Na doped ZnO nanocrystalline thin films synthesized using sol–gel spin coating technique

Sodium (Na) doped Zinc oxide (ZnO) thin films have been deposited on a glass substrate by the sol–gel spin coating method. Effect of doping with various percentages of Na at a particular annealing temperature of 500 °C is studied. The samples were characterized by X-ray diffraction (XRD), micro-photoluminescence, Raman and Polarized Raman spectroscopy. The X-ray diffraction and micro-Raman spectroscopy confirmed the presence of Na substitution in zinc oxide and the wurtzite structure of the lattice is retained. An enhancement of resonant Raman scattering processes as well as longitudinal optical phonon overtones up to the fifth order were observed in the micro Raman spectra. The similar values of depolarization ratios obtained from Polarized Raman studies recommend no change in the symmetry. Photoluminescence showed a strong emission peak in the near UV at 3.2 eV and negligible visible emission.     

Fully automated standard addition method for the quantification of 29 polar pesticide metabolites in different water bodies using LC-MS/MS

A reliable quantification by LC-ESI-MS/MS as the most suitable analytical method for polar substances in the aquatic environment is usually hampered by matrix effects from co-eluting compounds, which are unavoidably present in environmental samples. The standard addition method (SAM) is the most appropriate method to compensate matrix effects. However, when performed manually, this method is too labour- and time-intensive for routine analysis. In the present work, a fully automated SAM using a multi-purpose sample manager “Open Architecture UPLC®-MS/MS” (ultra-performance liquid chromatography tandem mass spectrometry) was developed for the sensitive and reliable determination of 29 polar pesticide metabolites in environmental samples. A four-point SAM was conducted parallel to direct-injection UPLC-ESI-MS/MS determination that was followed by a work flow to calculate the analyte concentrations including monitoring of required quality criteria. Several parameters regarding the SAM, chromatography and mass spectrometry conditions were optimised in order to obtain a fast as well as reliable analytical method. The matrix effects were examined by comparison of the SAM with an external calibration method. The accuracy of the SAM was investigated by recovery tests in samples of different catchment areas. The method detection limit was estimated to be between 1 and 10 ng/L for all metabolites by direct injection of a 10-μL sample. The relative standard deviation values were between 2 and 10 % at the end of calibration range (30 ng/L). About 200 samples from different water bodies were examined with this method in the Rhine and Ruhr region of North Rhine-Westphalia (Germany). Approximately 94 % of the analysed samples contained measurable amounts of metabolites. For most metabolites, low concentrations ≤0.10 μg/L were determined. Only for three metabolites were the concentrations in ground water significantly higher (up to 20 μg/L). In none of the examined drinking water samples were the health-related indication values (between 1 and 3 μg/L) for non-relevant metabolites exceeded.     

Comparison of Alcoholic Fermentation Performance of the Free and Immobilized Yeast on Water Hyacinth Stem Pieces in Medium with Different Glucose Contents

Ethanol fermentation with Saccharomyces cerevisiae cells was performed in medium with different glucose concentrations. As the glucose content augmented from 200 to 250 g/L, the growth of the immobilized cells did not change while that of the free cells was reduced. At higher glucose concentration (300, 350, and 400 g/L), the cell proliferation significantly decreased and the residual sugar level sharply augmented for both the immobilized and free yeast. The specific growth rate of the immobilized cells was 27–65 % higher than that of the free cells, and the final ethanol concentration in the immobilized yeast cultures was 9.7–18.5 % higher than that in the free yeast cultures. However, the immobilized yeast demonstrated similar or slightly lower ethanol yield in comparison with the free yeast. High fermentation rate of the immobilized yeast was associated with low unsaturation degree of fatty acids in cellular membrane. Adsorption of S. cerevisiae cells on water hyacinth stem pieces in the nutritional medium decreased the unsaturation degree of membrane lipid and the immobilized yeast always exhibited lower unsaturation degree of membrane lipid than the free yeast in ethanol fermentation.     

Dealing with a local heating effect when measuring catalytic solids in a reactor with Raman spectroscopy

In continuation of our previous work on the applicability of the G(R(infinity)) correction factor for the quantification of Raman spectra of coke during propane dehydrogenation experiments (Phys. Chem. Chem. Phys., 2005, 7, 211), research has been carried out on the potential of this correction factor for the quantification of supported metal oxides during reduction experiments. For this purpose, supported chromium oxide catalysts have been studied by combined in situ Raman and UV-Vis spectroscopy during temperature programmed reduction experiments with hydrogen as reducing agent. The goal was to quantify on-line the amount of Cr(6+) in a reactor based on the measured in situ Raman spectra. During these experiments, a significant temperature effect was observed, which has been investigated in more detail with a thermal imaging technique. The results revealed a temperature 'on the spot' that can exceed 100 degrees C. It implies that Raman spectroscopy can have a considerable effect on the local reaction conditions and explains observed inconsistencies between the in situ UV-Vis and Raman data. In order to minimize this heating effect, reduction of the laser power, mathematical matching of the spectroscopic data, a different cell design and a change in reaction conditions has been evaluated. It is demonstrated that increasing the reactor temperature is the most feasible method to solve the heating problem. Next, it allows the application of in situ Raman spectroscopy in a reliable quantitative way without the need of an internal standard.     

Ultra-Performance Liquid Chromatography with Electrospray Ionization Tandem Mass Spectrometry for the Determination of Ketoconazole in Anti-Dandruff Shampoo

A fast and highly sensitive method for the quantification of ketoconazole in antidandruff emulsion formulas was developed and validated. Sample preparation utilizing solid-phase extraction was a simple and reliable method for extracting both ketoconazole and its internal standard miconazole from the samples: 97 ± 3% for ketoconazole and 93 ± 4% for the internal standard. The separation by isocratic ultra-high performance liquid chromatography and multiple-stage mass spectrometry with a reversed-phase C₁₈ column was performed within 10 min. The method, which operated in a selective reaction monitoring mode specific to ketoconazole, was validated for quantitative use. The intra- and inter-day precision values were <5% and their accuracies ranged from 89.6 to 96.2%. The ketoconazole concentrations in two samples obtained by the established protocol were comparable to the concentrations indicated on the labels of the formulations. Thus, this paper describes the first use of ultra-high performance liquid chromatography and multiple-stage mass spectrometry for the determination of ketoconazole.     

Simultaneous determination of six hydrophilic ethers at trace levels using coconut charcoal adsorbent and gas chromatography/mass spectrometry

The main objective of the following study was to determine the efficiency of a method that uses coconut charcoal as a solid-phase extraction (SPE) adsorbent in order to simultaneously detect six hydrophilic ether species in water in the low microgram-per-liter range. The applied method was validated for quantification of ethyl tert-butyl ether, 1,4-dioxane, ethylene glycol dimethyl ether (monoglyme), diethylene glycol dimethyl ether (diglyme), triethylene glycol dimethyl ether (triglyme) and tetraethylene glycol dimethyl ether (tetraglyme). SPE followed by gas chromatography/mass spectrometry of the extracts using the selected ion monitoring mode allowed for establishing low detection limits in the range of 0.007–0.018 μg/L in ultrapure water and 0.004–0.020 μg/L in environmental samples. Examination of the method accuracy and precision resulted in a recovery greater than 86.8 % for each compound with a relative standard deviation of less than 6.6 %. A stability study established a 5-day holding time for the unpreserved water samples and extracts. Finally, 27 samples obtained from surface water bodies in Germany were analyzed for the six hydrophilic ethers. Each analyte was detected in at least eight samples at concentrations reaching 2.0 μg/L. The results of this study emphasize the advantage of the method to simultaneously determine six hydrophilic ether compounds. The outcome of the surface water analyses augments a concern about their frequent and significant presence in surface water bodies in Germany.     

A new ultrafast and high-throughput mass spectrometric approach for the therapeutic drug monitoring of the multi-targeted anti-folate pemetrexed in plasma from lung cancer patients

An analytical assay has been developed and validated for ultrafast and high-throughput mass spectrometric determination of pemetrexed concentrations in plasma using matrix assisted laser desorption/ionization–triple quadrupole–tandem mass spectrometry. Patient plasma samples spiked with the internal standard methotrexate were measured by multiple reaction monitoring. The detection limit was 0.4 fmol/μL, lower limit of quantification was 0.9 fmol/μL, and upper limit of quantification was 60 fmol/μL, respectively. Overall observed pemetrexed concentrations in patient samples ranged between 8.7 (1.4) and 142.7 (20.3)?pmol/μL (SD). The newly developed mass spectrometric assay is applicable for (routine) therapeutic drug monitoring of pemetrexed concentrations in plasma from non-small cell lung cancer patients.     

Quantification of BTEX in Soil by Headspace SPME–GC–MS Using Combined Standard Addition and Internal Standard Calibration

There is a great demand for simple, fast and accurate methods for quantification of volatile organic contaminants in soil samples. Solid-phase microextraction (SPME) has a huge potential for this purpose, but its application is limited by insufficient accuracy caused by a matrix effect. The aim of this research was to develop the method for BTEX quantification in soil using combined standard addition (SA) and internal standard (IS) calibration. Deuterated benzene (benzene-d6) was used as the internal standard for all analytes. The optimized method includes spiking replicate samples with different concentrations of BTEX standards and the same concentration of benzene-d6, equilibration of soil samples at 40 °C during 2 h, and SPME–GC–MS analysis. Precision and accuracy of IS and SA methods were compared on different soil matrices. Combined SA + IS method provided more precise calibration plots compared to the conventional SA calibration. The SA + IS calibration provided more precise and accurate results compared with a reference method based on solvent extraction followed by GC–MS when applied to BTEX quantification in real soil samples (spiked with diesel fuel and aged). Recoveries of BTEX from soil samples spiked with known concentrations of analytes using the developed method were in the range of 73–130% with RSD values less than 15% for all BTEX. The proposed simultaneous standard addition and internal standard approach can be advantageous and adopted for improved quantification of other toxic VOCs in soil.     

Highly Sensitive Determination of Butyl Xanthate in Surface and Drinking Water by Headspace Gas Chromatography with Electron Capture Detector

A highly sensitive and convenient method for the determination of butyl xanthate in surface water and drinking water was developed by headspace gas chromatography with electron capture detector (HS–GC–ECD). The analytical method was based on the decomposition of butyl xanthate under an acidic condition, generating carbon disulfide, which could be sensitively detected by gas chromatography with electron capture detector. The signal of CS₂ from the decomposition of potassium butyl xanthate was directly proportional to the concentration of potassium butyl xanthate over the range 0.7–100 ng/mL. The detection limit at a signal-to-noise ratio of three (S/N = 3) for potassium butyl xanthate was 0.3 ng/mL (~1.6 × 10⁻⁹ mol/L), which was more than two orders of magnitude lower than the popular UV methods and close to one order of magnitude lower than the similar headspace gas chromatography–mass spectroscopy method. The relative standard deviation (R.S.D.) within a day and in 3 days for potassium butyl xanthate at both 5 and 50 ng/mL was less than 4.7 %, suggesting good analytical performance of the present method. Good recoveries from 93.3 to 104.7 % were obtained from spiked surface and drinking water samples, indicating that the proposed HS–GC–ECD method was applicable for the quantification of butyl xanthate in surface and drinking water. Compared with other reported methods, the present method is highly sensitive, without sample preparation, and easily extended to the analysis of other xanthates.

     

Microextraction by packed sorbents combined with surface-enhanced Raman spectroscopy for determination of musk ketone in river water

Microextraction by packed sorbents (MEPS) combined with Surface-enhanced Raman spectroscopy (SERS) was investigated, and applied to the determination of musk ketone (MK) in river water samples. The full MEPS–SERS method includes analyte enrichment by MEPS preconcentration with C₁₈ sorbent followed by SERS detection supported by silver nanoparticles. An eluent drop containing the analyte is deposited directly from the MEPS syringe on a CaF₂ glass plate. When the drop has dried, a specific volume of silver nanoparticles solution is added on it before each SERS measurement. Several experimental variables were studied in depth; under the optimum experimental conditions MK can be extracted from a 500 μL sample with recoveries in the range 47–63 %. The limit of detection was 0.02 mg L^?1 and the relative standard deviation 15.2 % (n?=?4). Although not investigated in this work, the proposed method might be suitable for in-situ monitoring, because of the portability of the Raman spectrometer used.

Radon measurement in carbonated water with the Lucas cell and charcoal adsorption methods

There have been developed several different methods for measuring radon concentration in water which are now widely used, such as: liquid scintillation counting, Lucas cell counting, gamma and alpha spectroscopy. However, as far as the radon measurements in carbonated water are concerned, there are some issues caused by the gas excess. The aim of our work was to develop a simple method for measuring radon concentration in carbonated water that can be used for in situ measurements. Nevertheless, we propose not one, but two methods for measuring radon concentration in carbonated water. Thus, the first one is based on Lucas scintillation cells, and can be used for on-site measurements, while the second one utilizes activated charcoal adsorption, and needs a setup laboratory for gamma spectrometry measurements. For the evaluation of the methods, we compared the results of the Lucas cell-Luk3C method and of the activated charcoal method, both for non-carbonated and carbonated water. The simplest method for radon concentration determination—Lucas cell method—was successfully applied to fourteen natural carbonated water samples from Borsec to Bilbor area. The radon concentrations obtained ranged from 5.6 ± 0.5 to 39.6 ± 4.0 Bq/L, with a mean of 15.9 ± 2.6 Bq/L, these values are lower than 100 Bq/L, the maximum value recommended by the World Health Organization.     

Determination of Concentration Levels of Organochlorine Pesticides in Water from the Mandacaru Stream in Maringá-Paraná-Brazil Employing Gas Chromatography-Mass Spectrometry

In this work, a method to determine the concentration levels of organochlorine pesticides in water samples from the Mandacaru stream in the region of Maringá- Paraná was validated, using the technique of solid phase extraction associated with gas chromatography coupled to mass spectrometry. In the optimization of the method, parameters such as injector temperature and splitless time were evaluated. The analytical curves showed linear correlation values greater than 0.99 (R² > 0.99) for all compounds. The detection limits of 0.243 µg L^?1 to 1.200 µg L^?1 and quantification of 5.0 µg L^?1 were obtained for pesticides and the recovery values were between 88.25 and 127.3%. Values of relative standard deviation were less than 6.79%. In the water samples analyzed were found four organochlorine pesticides, two with concentrations within the limits set by national legislation and two with concentrations above these limits.     

A flow-through microarray cell for the online SERS detection of antibody-captured E. coli bacteria

We present an immunoassay microarray flow-through system for the surface-enhanced Raman scattering (SERS) analysis of bacteria. The system has been constructed to support and automatize the nondestructive in situ analysis of different microorganisms in aqueous environment. After the immobilization of the desired antibodies to an activated PEG-coated surface, the chip is placed into the flow cell which is then flushed with the contaminated sample. Finally, colloidal metal nanoparticles are added and the cells are detected label-free by SERS. Here, we introduce the successful imaging of single microorganisms in the flow cell as well as the quantification of microorganisms in water by SERS mapping with a linear range between 4.3 × 10³ to 4.3 × 10⁵ cells/mL. The method has potential for routine application, e.g. for drinking water control.