Your search keyword '"liquid-liquid extraction"' showing total 282 results

1. Quantification of Dehydroepiandrosterone, 17β-Estradiol, Testosterone, and Their Sulfates in Mouse Tissues by LC-MS/MS.

Author

Yoo, Hong and Napoli, Joseph

Subjects

Animals, Chromatography, Liquid, Dehydroepiandrosterone, Estradiol, Female, Limit of Detection, Liquid-Liquid Extraction, Male, Mice, Inbred C57BL, Sulfuric Acid Esters, Tandem Mass Spectrometry, Testosterone

Abstract

We report a high-performance, liquid chromatography/tandem mass spectrometry (HPLC-MS/MS) assay to quantify without derivatizaton dehyroepiandrosterone (DHEA), 17β-estradiol (E2), testosterone (T), and their sulfates in serum and tissues. This assay functions well with multiple adipose depots, a previously unattained analysis. To delipidate and facilitate recovery, tissues were homogenized in acetonitrile, and the homogenate was frozen. The supernatant was evaporated, resuspended in an aqueous acetate buffer, and extracted with hexane to separate free (unconjugated) from sulfated steroids. Sulfated steroids in the aqueous medium were then hydrolyzed with sulfatase and extracted with hexane. Each extract was analyzed separately. HPLC resolution combined with the sensitivity and specificity of MS/MS allowed quantification of DHEA, E2, and T with 10, 10, and 5 fmol lower limits of quantification and linear ranges to 1 pmol. Application of the method to mouse serum and tissues reveals ranges of DHEA, E2, and T and their sulfates, and tissue-specific differences in steroid profile, especially white versus brown adipose. In addition, marginal decreases of T in all tissues and considerable increases in DHEA in male iWAT and eWAT in response to a high-fat diet further strengthen the inference regarding the role of steroid metabolism in adipogenesis. This assay permits detailed studies of interactions between adiposity and sex steroids in serum and tissues, including adipose.

Published

2019

2. Better Together: Tandem Mass Spectrometry Achieves up to 50 Times Lower Quantification of 62 Disinfection Byproducts in Drinking Water.

Author

Justen PT, Beavers CA, Forster ALB, and Richardson SD

Subjects

Disinfectants analysis, Liquid-Liquid Extraction, Humans, Tandem Mass Spectrometry methods, Drinking Water analysis, Drinking Water chemistry, Water Pollutants, Chemical analysis, Disinfection, Gas Chromatography-Mass Spectrometry methods

Abstract

Disinfection byproducts (DBPs) are ubiquitous contaminants present in nearly all drinking water and are associated with adverse health effects in human epidemiologic studies. The most toxic DBPs are unregulated and often occur at concentrations well below regulated DBPs; thus, quantification at low parts-per-trillion (ng/L) levels is critical in assessing exposure. We developed a new liquid-liquid extraction-gas chromatography-tandem mass spectrometry (LLE-GC-MS/MS) method with the first analysis by tandem gas chromatography-mass spectrometry of 23 priority unregulated DBPs including 13 haloacetamides, 3 haloacetic acids, 2 haloacetonitriles, 1 haloacetaldehyde, 2 haloketones, and 2 halonitromethanes. When combined with our previous GC-MS/MS method for haloacetic acids and previously reported MS/MS transitions that we optimized for this method, the analysis of 62 regulated and priority unregulated DBPs at lower quantification limits is achieved. Limits of quantification for most DBPs were between 5 and 30 ng/L with r 2 > 0.99 and an average of 9 times lower limits of quantification (LOQs) compared to LLE-GC-MS using selected ion monitoring (SIM). Relative standard deviations ranged from 0.7 to 30% for 61 DBPs in spiked samples. This new method was validated using tap waters from four US cities, where individual DBP concentrations ranged from 5 to 126,882 ng/L. This project provides the most comprehensive GC-MS/MS method for DBP analysis to date and is capable of analyzing volatile and semivolatile DBPs across nine different compound classes, including a class not previously analyzed by GC-MS/MS.

Published

2024

3. Rapid Sample Pretreatment Facilitating SERS Detection of Trace Weak Organic Acids/Bases in Complex Matrices.

Author

Xu J, Zhang S, Luo SH, Xiong CR, Zhu M, Chang J, Zou B, Ren B, Tian ZQ, and Liu GK

Subjects

Liquid-Liquid Extraction, Humans, Pentacyclic Triterpenes, Food Analysis methods, Metal Nanoparticles chemistry, Spectrum Analysis, Raman methods, Solid Phase Extraction

Abstract

Fast and efficient sample pretreatment is the prerequisite for realizing surface-enhanced Raman spectroscopy (SERS) detection of trace targets in complex matrices, which is still a big issue for the practical application of SERS. Recently, we have proposed a highly performed liquid-liquid extraction (LLE)-back extraction (BE) for weak acids/bases extraction in drinking water and beverage samples. However, the performance efficiency decreased drastically on facing matrices like food and biological blood. Based on the total interaction energies among target, interferent, and extractant molecules, solid-phase extraction (SPE) with a higher selectivity was introduced in advance of LLE-BE, which enabled the sensitive (μg L -1 level) and rapid (within 10 min) SERS detection of both koumine (a weak base) and celastrol (a weak acid) in different food and biological samples. Further, the high SERS sensitivity was determined unmanned by Vis-CAD (a machine learning algorithm), instead of the highly demanded expert recognition. The generality of SPE-LLE-BE for various weak acids/bases (2 < p K a < 12), accompanied by the high efficiency, easy operation, and low cost, offers SERS as a powerful on-site and efficient inspection tool in food safety and forensics.

Published

2024

4. Rapid Sample Pretreatment Facilitating SERS Detection of Trace Weak Organic Acids/Bases in Simple Matrices.

Author

Xu J, Xie L, Zhu M, Xiong C, Huang Q, Zhang M, Ren B, Tian Z, and Liu G

Subjects

Beverages, Liquid-Liquid Extraction, Spectrum Analysis, Raman methods, Drinking Water

Abstract

Surface-enhanced Raman spectroscopy (SERS) is a powerful tool for highly sensitive qualitative and quantitative analyses of trace targets. However, sensitive SERS detection can only be facilitated with a suitable sample pretreatment in fields related to trace amounts for food safety and clinical diagnosis. Currently, the sample pretreatment for SERS detection is normally borrowed and improved from the ones in the lab, which yields a high recovery but is tedious and time-consuming. Rapid detection of trace targets in a complex environment is still a considerable issue for SERS detection. Herein, we proposed a liquid-liquid extraction method coupled with a back-extraction method for sample pretreatment based on the pH-sensitive reversible phase transition of the weak organic acids and bases, where the lowest detectable concentrations were identical before and after the pretreatment process. The sensitive (μg L -1 level) and rapid (within 5 min) SERS detection of either koumine, a weak base, or celastrol, a weak acid, was demonstrated in different drinking water samples and beverages. Furthermore, target generality was demonstrated for a variety of weak acids and bases (2 < p K a < 12), and the hydrophilicity/hydrophobicity of the target determines the pretreatment efficiency. Therefore, the LLE-BE coupled SERS was developed as an easy, rapid, and low-cost tool for the trace detection of the two types of targets in simple matrices, which paved the way toward trace targets in complex matrices.

Published

2024

5. Multielement Determination of Trace Heavy Metals in Water by Microwave-Induced Plasma Atomic Emission Spectrometry after Extraction in Unconventional Single-Salt Aqueous Biphasic System.

Author

Smirnova, Svetlana V., Samarina, Tatiana O., Ilin, Dmitry V., and Pletnev, Igor V.

Subjects

*HEAVY metal content of water, *ATOMIC emission spectroscopy, *LIQUID-liquid extraction, *ORGANIC solvents, *RESORCINOL

Abstract

For the first time liquid-liquid extraction was used for the preconcentration of heavy metals prior to their determination in water by microwave-induced plasma atomic emission spectrometry (MP-AES). Extraction of Pb(II), Cd(II), Co(II), Ni(II), Zn(II), and Cu(II) was performed in unconventional aqueous biphasic system (ABS) formed by addition of hydrophobic solid salt, namely, tetrahexylammonium bromide, to aqueous sample, with neither organic solvents nor salting-out agents being used. The metal ions were quantitatively recovered with 4-(2-pyridylazo)-resorcinol (PAR). The extract was diluted with ethanol/HCl and introduced directly into an MP-AES instrument. The factors influencing extraction (pH, reagent concentration, phase contact time, etc.) and MP-AES detection parameters were studied and optimized. For the developed method, limits of detection of 1.3, 4.9, 0.06, 1.2, 4.2, and 3.2 µg L-1 were obtained for cadmium, cobalt, copper, nickel, lead, and zinc, respectively, providing from 60- to 500-fold improvement as compared with the analysis without preconcentration. The method was applied for the analysis of two certified reference materials (CRM) of wastewater and surface water as well as the samples of well and seawater. Coupling MP-AES with ABS extraction significantly extends the capabilities of the method, especially for the analysis of high salinity waters. [ABSTRACT FROM AUTHOR]

Published

2018

6. Rapid Sample Preparation Using Slug Flow–Laminar Flow: Passive In Situ Microextraction/Stripping Coupling

Author

Qiang Zheng, Cong Xu, Tao Wang, Wensheng Wang, and Yu Ma

Subjects

Chromatography, Liquid Phase Microextraction, Chemistry, Liquid-Liquid Extraction, Extraction (chemistry), Water, Laminar flow, Slug flow, Stripping (fiber), Analytical Chemistry, Membrane, Liquid–liquid extraction, Mass transfer, Sample preparation

Abstract

To increase the detection accuracy of radioactive samples, sample preparation through liquid-liquid extraction (LLE) before instrumental analysis is a crucial step. LLE preparation involves multiple steps including the tedious separation steps of co-extraction and stripping, which may cause sample loss, radioactive contamination, and radioactive leaks. In this study, a novel hybrid slug flow-laminar flow (SFLF) microchip in passive mode was designed to couple extraction and stripping in situ to realize a one-step sample preparation. The difficulty in maintaining stable water-organic-water interfaces was mitigated by using a partition wall and three resistance isolation areas. The mass transfer performance of the SFLF microchip was investigated and compared with that of the supported liquid membrane and three-layer laminar flow microextraction/stripping systems. Furthermore, the applicability of the SFLF system in preparing radioactive samples was validated through the selective separation of Ce and Pr from Cs and Sr. The novel SFLF microextraction/stripping system has a stable flow pattern, high mass transfer efficiency, and superior operating flexibility.

Published

2021

7. Molecular Comparison of Solid-Phase Extraction and Liquid/Liquid Extraction of Water-Soluble Petroleum Compounds Produced through Photodegradation and Biodegradation by FT-ICR Mass Spectrometry

Author

Gregory T. Blakney, Amy M. McKenna, Chad R. Weisbrod, and Huan Chen

Subjects

chemistry.chemical_classification, Photolysis, Chromatography, Electrospray ionization, Solid Phase Extraction, 010401 analytical chemistry, Extraction (chemistry), Water, Biodegradation, 010402 general chemistry, Mass spectrometry, 01 natural sciences, Mass Spectrometry, Fourier transform ion cyclotron resonance, 0104 chemical sciences, Analytical Chemistry, Petroleum, Hydrocarbon, chemistry, Liquid–liquid extraction, Solid phase extraction

Abstract

We apply two widely used extraction techniques, liquid/liquid extraction and solid-phase extraction with styrene-divinylbenzene polymer with a proprietary nonpolar surface priority pollutant (PPL) to water-soluble compounds generated through photodegradation and biodegradation of petroleum. We compare the molecular composition of bio- and photodegraded water-soluble organic (WSO) acids by 21 T negative-ion electrospray ionization Fourier transform ion cyclotron resonance mass spectrometry (FT-ICR MS). We highlight the compositional differences between the two extraction techniques for abiotic and biotic degradation processes and identify known toxic species (naphthenic acids) produced through hydrocarbon biodegradation identified by liquid/liquid extraction (LLE) that are not detected with solid-phase extraction (SPE) of the same sample. Photodegraded WSO compounds extracted by SPE-PPL correspond to species with higher O/C ratio and carbon number compared to LLE extracted compounds. Naphthenic acids, a recalcitrant class of nonaromatic carboxylic acids and known acute toxicants formed through biodegradation of oil, are detected in LLE extracts (up to C30 and double-bond equivalents, DBE < 3) but are not detected in SPE-PPL extracts. This suggests that LLE and SPE-PPL retain different water-soluble oil species based on the dominant type of oil weathering process.

Published

2021

8. Generic Enrichment of Organic Contaminants in Human Biomonitoring: Application in Monitoring Early Life Exposures to Fipronil via Breast Milk

Author

Zhibin Liu, Dawei Chen, Bing Lyu, Jingguang Li, Yunfeng Zhao, and Yongning Wu

Subjects

Milk, Human, Liquid-Liquid Extraction, Humans, Pyrazoles, Female, Analytical Chemistry, Biological Monitoring

Abstract

In human biomonitoring, a high-throughput extraction and enrichment method for multiple types of organic contaminants at the part-per-trillion level is critical yet challenging, especially in the limited sample volume. When large-scale sample analysis is involved, low cost is often what we should consider. We describe a generic and straightforward cold-induced liquid-liquid extraction (CI-LLE) strategy to meet this need. Current methods for extracting and enriching organic contaminants from biological samples often require multistep sample processing, including specially tailoring the extraction solvent or adsorbents. This method uses cold-induced phase separation to achieve the extraction and enrichment of studied organic contaminants by adjusting the proportion of acetonitrile/water mixture, so as to integrate the extraction and enrichment in one step without additional reagents and adsorbents. In this study, fipronil insecticide was used as a representative compound to determine the key parameters of CI-LLE. The optimized CI-LLE procedure allowed simultaneous extraction and enrichment of studied organic contaminants, providing excellent enrichment factors (especially for lipophilic organic contaminants). CI-LLE was further applied in monitoring early life exposures of fipronil in 109 breast milk samples. This study provided baseline data on fipronil levels in breast milk samples from China. For infants, exposure to fipronil is of concern. In summary, CI-LLE provides a feasible solution for a generic, efficient, and low-cost preparation of biological samples and promotes high-throughput batch analysis of organic contaminants for large-scale human biomonitoring.

Published

2022

9. Fully Automatic In-Syringe Magnetic Stirring-Assisted Dispersive Liquid-Liquid Microextraction Hyphenated to High-Temperature Torch Integrated Sample Introduction System-Inductively Coupled Plasma Spectrometer with Direct Injection of the Organic Phase.

Author

Sánchez, Raquel, Horstkotte, Burkhard, Fikarová, Katerina, Sklenárová, Hana, Maestre, Salvador, Miró, Manuel, and Todolí, Jose-Luis

Subjects

*LIQUID-liquid extraction, *HIGH temperatures, *INDUCTIVELY coupled plasma spectrometry, *ATOMIZERS, *MIXING

Abstract

A proof of concept study involving the online coupling of automatic dispersive liquid-liquid microextraction (DLLME) to inductively coupled plasma optical emission spectrometry (ICP OES) with direct introduction and analysis of the organic extract is herein reported for the first time. The flow-based analyzer features a lab-in-syringe (LIS) setup with an integrated stirring system, a Meinhard nebulizer in combination with a heated single-pass spray chamber, and a rotary injection valve, used as an online interface between the microextraction system and the detection instrument. Air-segmented flow was used for delivery of a fraction of the nonwater miscible extraction phase, 12 µL of xylene, to the nebulizer. All sample preparative steps including magnetic stirring assisted DLLME were carried out inside the syringe void volume as a size-adaptable yet sealed mixing and extraction chamber. Determination of trace level concentrations of cadmium, copper, lead, and silver as model analytes has been demonstrated by microextraction as diethyldithiophosphate (DDTP) complexes. The automatic LIS-DLLME method features quantitative metal extraction, even in troublesome sample matrixes, such as seawater, salt, and fruit juices, with relative recoveries within the range of 94-103%, 93-100%, and 92-99%, respectively. Furthermore, no statistically significant differences at the 0.05 significance level were found between concentration values experimentally obtained and the certified values of two serum standard reference materials. [ABSTRACT FROM AUTHOR]

Published

2017

10. RapidFire Mass Spectrometry with Enhanced Throughput as an Alternative to Liquid-Liquid Salt Assisted Extraction and LC/MS Analysis for Sulfonamides in Honey.

Author

Veach, Brian T., Mudalige, Thilak K., and Rye, Peter

Subjects

*MASS spectrometry, *LIQUID-liquid extraction, *SALT, *LIQUID chromatography-mass spectrometry, *SULFONAMIDES, *HONEY analysis

Abstract

The use of veterinary drugs in honey bees for the prevention of infectious disease is ever increasing due to the spread of colony collapse disorder around the world. The United States Food and Drug Administration is concerned about the presence of these drugs residues in honey as they often lead to health concerns or potential antibiotic resistance. Currently there is a need for a rapid screening method for the detection of veterinary drugs in honey. Herein is a method that utilizes automated solid-phase extraction that is directly coupled to a mass spectrometer for the quantitative screening of 12 different regulated sulfonamides in honey. Identification of the residues was performed using tandem mass spectrometry (MS/MS) with a triple quadrupole mass spectrometer. The acquisition method developed for this analysis can extract with the automated solid-phase extraction system and analyze a single sample on the mass spectrometer in approximately 20 s, with minimal sample preparation. A target testing limit of 10 ng/g in honey for the sulfonamides was used based upon action limits set for other food commodities regulated by the United States Food and Drug Administration. A complete method validation procedure was conducted to evaluate the effectiveness of this quantitative screening method. [ABSTRACT FROM AUTHOR]

Published

2017

11. Trace Analysis of 61 Emerging Br-, Cl-, and I-DBPs: New Methods to Achieve Part-Per-Trillion Quantification in Drinking Water

Author

Susana Y. Kimura, Alena Bensussan, Joshua M. Allen, Hannah K. Liberatore, Susan D. Richardson, and Amy A. Cuthbertson

Subjects

Bromides, Haloacetic acids, Liquid-Liquid Extraction, 010402 general chemistry, 01 natural sciences, Analytical Chemistry, chemistry.chemical_compound, Chlorides, Tap water, Polysaccharides, medicine, Selected ion monitoring, Solid phase extraction, Derivatization, Quadrupole mass analyzer, Detection limit, Chromatography, Drinking Water, Solid Phase Extraction, 010401 analytical chemistry, Selected reaction monitoring, Iodides, 0104 chemical sciences, chemistry, Water Pollutants, Chemical, medicine.drug

Abstract

Disinfection byproducts (DBPs) are a ubiquitous source of chemical exposure in drinking water and have been associated with serious health impacts in human epidemiologic studies. While toxicology studies have pinpointed DBPs with the greatest toxic potency, analytical methods have been lacking for quantifying complete classes of most toxic DBPs at sufficiently low quantification limits (ng/L). This new method reports the parts-per-trillion quantification for 61 toxicologically significant DBPs from 7 different chemical classes, including unregulated iodinated haloacetic acids (HAAs) and trihalomethanes (THMs), haloacetaldehydes, haloketones, haloacetonitriles, halonitromethanes, and haloacetamides, in addition to regulated HAAs and THMs. The final optimized method uses salt-assisted liquid-liquid extraction in a single extraction method for a wide range of DBPs, producing the lowest method detection limits to-date for many compounds, including highly toxic iodinated, brominated, and nitrogen-containing DBPs. Extracts were divided for the analysis of the HAAs (including iodinated HAAs) by diazomethane derivatization and analysis using a GC-triple quadrupole mass spectrometer with multiple reaction monitoring, resulting in higher signal-to-noise ratios, greater selectivity, and improved detection of these compounds. The remaining DBPs were analyzed using a GC-single quadrupole mass spectrometer with selected ion monitoring, utilizing a multimode inlet allowed for lower injection temperatures to allow the analysis of thermally labile DBPs. Finally, the use of a specialty-phase GC column (Restek Rtx-200) significantly improved peak shapes, which improved separations and lowered detection limits. Method detection limits for most DBPs were between 15 and 100 ng/L, and relative standard deviations in tap water samples were mostly between 0.2 and 30%. DBP concentrations in real samples ranged from 40 to 17 760 ng/L for this study.

Published

2020

12. A Novel Approach for the Determination of the Ge Isotope Ratio Using Liquid-Liquid Extraction and Hydride Generation by Multicollector Inductively Coupled Plasma Mass Spectrometry

Author

Ludwik Halicz, Ewa Bulska, Andrii Tupys, and Jakub Karasiński

Subjects

Isotope, Chemistry, Hydride, Spectrum Analysis, Extraction (chemistry), Liquid-Liquid Extraction, Analytical chemistry, chemistry.chemical_element, Germanium, Mass Spectrometry, Article, Analytical Chemistry, Isotopic ratio, Isotopes, Liquid–liquid extraction, Sensitivity (control systems), Inductively coupled plasma mass spectrometry

Abstract

In this work, a method for the accurate and precise determination of the Ge isotope ratio in synthetic water and natural samples of geological origin using multicollector inductively coupled plasma mass spectrometry (MC-ICPMS) with hydride generation was developed. The method was based on the liquid-liquid extraction of Ge to eliminate all elements affecting the generation of germanium hydrides. The standard-sample bracketing method was used to correct instrumental bias. Registration of analytical signal in time-resolved mode gave way to choose signals with best parameters and improved the precision of the results. Controlling the pH by using acetic buffer boosted the sensitivity by nearly five times in comparison to hydride generation methods suggested by other authors. The newly developed method is much simpler and quicker, does not need laborious Ge separation with ion-exchange resins, and thanks to its superior sensitivity, allows measurements of the Ge isotopic ratio in materials with relatively low Ge content. Delta values of the 74Ge/70Ge isotope ratio were measured in standard reference materials for which reference values were available in the GeoREM database. We demonstrated that the accuracy and precession of this method are equally good or better than methods proposed by other authors.

Published

2021

13. Chemical Isotope Labeling LC-MS for High Coverage and Quantitative Profiling of the Hydroxyl Submetabolome in Metabolomics.

Author

Shuang Zhao, Xian Luo, and Liang Li

Subjects

*HYDROXYL group, *METABOLOMICS, *ACTIVATION (Chemistry), *LIQUID chromatography-mass spectrometry, *LIQUID-liquid extraction

Abstract

A key step in metabolomics is to perform accurate relative quantification of the metabolomes in comparative samples with high coverage. Hydroxyl-containing metabolites are an important class of the metabolome with diverse structures and physical/chemical properties; however, many of them are difficult to detect with high sensitivity. We present a high-performance chemical isotope labeling liquid chromatography mass spectrometry (LC-MS) technique for in-depth profiling of the hydroxyl submetabolome, which involves the use of acidic liquid--liquid extraction to enrich hydroxyl metabolites into ethyl acetate from an aqueous sample. After drying and then redissolving in acetonitrile, the metabolite extract is labeled using a base-activated 12C- or I3Cdansylation reaction. A fast step-gradient LC-UV method is used to determine the total concentration of labeled metabolites. On the basis of the concentration information, a 12C-labeled individual sample is mixed with an equal mole amount of a 13C-labeled pool or control for relative metabolite quantification. The 12C-/13C-labeled mixtures are individually analyzed by LC-MS, and the resultant peak pairs of labeled metabolites in MS are measured for relative quantification and metabolite identification. A standard library of 85 hydroxyl compounds containing MS, retention time, and MS/MS information was constructed for positive metabolite identification based on matches of two or all three of these parameters with those of an unknown. Using human urine as an example, we analyzed samples of 1:1 12C-/13C-labeled urine in triplicate with triplicate runs per sample and detected an average of 3759 ± 45 peak pairs or metabolites per run and 3538 ±71 pairs per sample with 3093 pairs in common (n = 9). Out of the 3093 peak pairs, 2304 pairs (75%) could be positively or putatively identified based on metabolome database searches, including 20 pairs positively identified using the dansylated hydroxyl standards library. The majority of detected metabolites were those containing hydroxyl groups. This technique opens a new avenue for the detailed characterization of the hydroxyl submetabolome in metabolomics research. [ABSTRACT FROM AUTHOR]

Published

2016

14. Miniscale Liquid-Liquid Extraction Coupled with Full Evaporation Dynamic Headspace Extraction for the Gas Chromatography/Mass Spectrometric Analysis of Polycyclic Aromatic Hydrocarbons with 4000-to-14 000-fold Enrichment.

Author

Shu Min Liew, Christina, Xiao Li, and Hian Kee Lee

Subjects

*POLYCYCLIC aromatic hydrocarbons, *LIQUID-liquid extraction, *EVAPORATION (Chemistry), *GAS chromatography/Mass spectrometry (GC-MS), *CHEMICAL sample preparation, *AQUEOUS solutions

Abstract

A new sample preparation approach of combining a miniscale version of liquid-liquid extraction (LLE), termed miniscale-LLE (msLLE), with automated full evaporation dynamic headspace extraction (FEDHS) was developed. Its applicability was demonstrated in the extraction of several polycyclic aromatic hydrocarbons (PAHs) (acenaphthylene, acenaphthene, fluorene, phenanthrene, anthracene, fluoranthene, and pyrene) from aqueous samples. In the first step, msLLE was conducted with 1.75 mL of n-hexane, and all of the extract was vaporized through a Tenax TA sorbent tube via a nitrogen gas flow, in the FEDHS step. Due to the stronger π-π interaction between the Tenax TA polymer and PAHs, only the latter, and not n-hexane, was adsorbed by the sorbent. This selectivity by the Tenax TA polymer allowed an effective concentration of PAHs while eliminating n-hexane by the FEDHS process. After that, thermal desorption was applied to the PAHs to channel them into a gas chromatography/mass spectrometric (GC/MS) system for analysis. Experimental parameters affecting msLLE (solvent volume and mixing duration) and FEDHS (temperature and duration) were optimized. The obtained results achieved low limits of detection (1.85-3.63 ng/L) with good linearity (r² > 0.9989) and high enrichment factors ranging from 4200 to 14 100. The optimized settings were applied to the analysis of canal water sampled from an industrial area and tap water, and this methodology was compared to stir-bar sorptive extraction (SBSE). This innovative combined extraction-concentration approach proved to be fast, effective, and efficient in determining low concentrations of PAHs in aqueous samples. [ABSTRACT FROM AUTHOR]

Published

2016

15. Baseline-Corrected Second-Order Derivative Electroanalysis Combined With Ultrasound-Assisted Liquid-Liquid Microextraction: Simultaneous Quantification of Fluoroquinolones at Low Levels.

Author

de Oliveira, Luiz Henrique and Gonçalves Trindade, Magno Aparecido

Subjects

*FLUOROQUINOLONES, *LIQUID-liquid extraction, *ELECTROCHEMICAL analysis, *CHEMICAL derivatives, *CARBON nanofibers, *WATER sampling

Abstract

A baseline-corrected second-order derivative procedure and a miniaturized sample preparation based on low-density solvent and ultrasound-assisted liquid-liquid microextraction (LDS-UA-LLME) was combined to provide the simultaneous electroanalysis of three fluoroquinolones (FQ) as emerging contaminants (ECs). The enhanced mathematical processing provided the best separation with an accurate measurement of the overlapping peaks during the simultaneous electro-oxidation of target FQs that were directly dropped on the surface of carbon nanofiber-modified screen-printed electrodes. The adapted LDS-UA-LLME protocol was the key step involved in the sample preparation, which preconcentrate target analytes from diluted tap water samples with an enrichment factor of around 80?, allowing their quantification at trace levels. This combined feature demonstrated the unique application of an electroanalytical technique for the simultaneous electroanalysis of three FQs in spiked tap water samples, with recovery values remarkably close to 100%. [ABSTRACT FROM AUTHOR]

Published

2016

16. Microfluidic System Enabling Multistep Tuning of Extraction Time Periods for Kinetic Analysis of Droplet-Based Liquid-Liquid Extraction.

Author

Natsuki Nakajima, Masumi Yamada, Shunta Kakegawa, and Minoru Seki

Subjects

*MICROFLUIDIC analytical techniques, *EXTRACTION (Chemistry), *LIQUID-liquid extraction, *KINETIC theory of liquids, *PHASE separation, *HYDRODYNAMICS, *MASS transfer

Abstract

When analyzing the kinetics of liquid--liquid extraction (LLE), the change in the concentration of extracted target molecules over time should be monitored for a known interfacial area. Herein, we developed a microfluidic system for precisely analyzing the kinetics of LLE using droplets of a constant size even in the presence of additives. Extraction is initiated by exchanging the carrier fluid for the droplets with a target solution and then terminated by phase separation, based on the principle of hydrodynamic filtration. By using one out of several pairs of outlet/buffer inlet at a given time, the extraction time period is tuned stepwise without changing the flow rate condition. We successfully demonstrated droplet-based LLE by controlling the extraction period from ~0.03 to ~1.2 s and evaluated the extraction kinetics of rhodamine B from the continuous aqueous phase to droplets of 1-octanol with a diameter of ~40 µm. In addition, the effect of additives on extraction efficiency was evaluated. The system presented in this study would be useful for determining rate constants for interfacial mass transfer in general LLE. kinetic studies as well as for developing new extraction chemistries and optimizing microfluidic chemical/ biochemical analysis systems that involve an LLE process. [ABSTRACT FROM AUTHOR]

Published

2016

17. Direct Biofluid Analysis Using Hydrophobic Paper Spray Mass Spectrometry.

Author

Damon, Deidre E., Davis, Kathryn M., Moreira, Camila R., Capone, Patricia, Cruttenden, Riley, and Badu-Tawiah, Abraham K.

Subjects

*MASS spectrometry, *LIQUID-liquid extraction, *ORGANIC compounds, *ORGANIC solvents, *ELECTROSTATIC atomization, *POINT-of-care testing

Abstract

Ambient electrostatic paper spray ionization from a hydrophobic paper occurs when a DC potential is applied to the dry paper triangle. Online liquid/liquid extraction of small organic compounds from a drop of biological fluid present on the dry hydrophobic paper is achieved with an organic spray solvent in under 1 min and utilizes in situ electrostatic-spray ionization for more efficient detection of extracted molecules. Direct analysis of small volumes of biofluids with no sample pretreatment is possible, which is applicable in point-of-care analyses. High sensitivity and quantitative accuracy was achieved for the direct analysis of illicit drugs in 4 µL of raw blood, serum, and whole urine. The study was extended to monitor the activity of alanine transaminase enzyme, a key biomarker for the detection of liver injury in patients (with HIV and tuberculosis) who typically take several medications at once. [ABSTRACT FROM AUTHOR]

Published

2016

18. Proteinase K Combining Two-Step Liquid–Liquid Extraction for Plasma Untargeted Liquid Chromatography–Mass Spectrometry-Based Metabolomics To Discover the Potential Mechanism of Colorectal Adenoma

Author

Qisong Zhang, Lingzhi Gong, Yanying Nong, and Zhongqiu Liu

Subjects

Adenoma, Adult, Male, Spectrometry, Mass, Electrospray Ionization, Gastrointestinal Diseases, Metabolite, Liquid-Liquid Extraction, 010402 general chemistry, 01 natural sciences, Analytical Chemistry, Plasma, chemistry.chemical_compound, Metabolomics, Liquid chromatography–mass spectrometry, Metabolome, Humans, Protein precipitation, Sample preparation, Chromatography, High Pressure Liquid, Chromatography, biology, 010401 analytical chemistry, Extraction (chemistry), Reproducibility of Results, Middle Aged, Proteinase K, 0104 chemical sciences, chemistry, biology.protein, Female, Endopeptidase K, Blood Chemical Analysis

Abstract

LC-MS-based untargeted metabolomics have been proven to be an extremely promising technique to discover biomarkers and explore the mechanisms underlying diseases, which, however, relies heavily on sample pretreatment for metabolite extraction. In the present study, a systematic and pragmatic evaluation of eight protocols employing conventional metabolites extraction strategies, protein precipitation (PPT), and liquid-liquid extraction (LLE), with and without proteinase K (PK) incubation, was performed simultaneously, using human plasma and a mixture of 39 endogenous metabolite standards. These protocols were as follows: (1) PPT with methanol, (2) PPT with acetonitrile, (3) PPT with 2-propanol, (4) two-step LLE of CH2Cl2-MeOH, followed by MeOH-H2O, (5) PK incubation combining two-step LLE of CH2Cl2-MeOH followed by MeOH-H2O, (6) two-step LLE of CHCl3-MeOH, followed by MeOH-H2O, (7) PK incubation combining two-step LLE of CHCl3-MeOH, followed by MeOH-H2O, (8) PK incubation combining MeOH-EtOH PPT. The results suggested that two-step LLE produced broader metabolome coverage than protein precipitation, and the addition of proteinase K enhanced the extraction performance further. Taken together, PK incubation combining two-step LLE of CHCl3-MeOH, followed by MeOH-H2O, was determined to be the most suitable extraction method, because of its broad metabolome coverage, high reproducibility, and satisfactory recovery. Next, the developed optimal sample preparation method was applied successfully to profile the plasma metabolome of colorectal adenoma and uncover its potential mechanism for significant differential changes in linoleic acid and phospholipid metabolism.

Published

2019

19. Implementation and Performance of the Gas Chromatography/Combustion/Isotope Ratio Mass Spectrometry-Based Method for the Confirmatory Analysis of Endogenous Anabolic Steroids during the Rio de Janeiro Olympic and Paralympic Games 2016

Author

Alessandro Casilli, Thais R. Silva, Gutierri Ricardo Dos Santos Gonçalves Salgueiro, Monica Costa Padilha, Fábio Azamor de Oliveira, Cristiane A. da Silva, Thomas Piper, Marco Aurélio Dal Sasso, Henrique Pereira, Raquel V.S. Silva, Francisco Radler de Aquino Neto, and Mario Thevis

Subjects

Anabolism, Estranes, Metabolite, Liquid-Liquid Extraction, 010402 general chemistry, Combustion, 01 natural sciences, Gas Chromatography-Mass Spectrometry, Analytical Chemistry, chemistry.chemical_compound, medicine, Humans, Testosterone, Sample preparation, Solid phase extraction, Isotope-ratio mass spectrometry, Testosterone Congeners, Chromatography, High Pressure Liquid, Doping in Sports, Carbon Isotopes, Chromatography, Chemistry, Solid Phase Extraction, 010401 analytical chemistry, Reproducibility of Results, Acetylation, Boldenone, 0104 chemical sciences, Gas chromatography, Brazil, Sports, medicine.drug

Abstract

Carbon isotope ratio (CIR) confirmation is one of the most complex and delicate analyses in the doping control field, due to the nature of the molecules to be confirmed, normally present in urinary samples as a consequence of an endogenous production. The requirements for method validation established by the World Anti-Doping Agency (WADA) have been pushing the accredited laboratories to improve their methods. The choice of the method is always a cost benefit ratio involving a hard-working and time-consuming analysis and the guarantee of reporting of reliable results. This work presents the method fully validated by the Brazilian Doping Control Laboratory as part of the preparation for the Rio de Janeiro Summer Olympic and Paralympic Games 2016. Sample preparation encompassed solid-phase extraction, liquid-liquid extraction, enzymatic hydrolysis, acetylation, and purification by preparative high-performance liquid chromatography, and analyses were performed by gas chromatography/combustion/isotope ratio mass spectrometry. This proved to be a robust method to CIR confirmation in a big event, as demonstrated by the analysis of 179 samples during the Games 2016, from clearly negative results and adverse findings for testosterone (T) and related substances, boldenone and its metabolite, 19-norandrosterone and formestane. Two atypical findings were also reported for T and metabolites.

Published

2019

20. Secreted Metabolome of Human Macrophages Exposed to Methamphetamine

Author

Akou Vei, Katarzyna Lech, Howard S. Fox, Spencer Jaquet, Sarah Zieschang, Pawel Ciborowski, Emma Harwood, Fang Yu, Sydney Burch, Brenda Morsey, and Katarzyna Pawlak

Subjects

Chemokine, Metabolite, Liquid-Liquid Extraction, 010402 general chemistry, 01 natural sciences, Article, Mass Spectrometry, Methamphetamine, Analytical Chemistry, chemistry.chemical_compound, Metabolomics, medicine, Metabolome, Humans, Innate immune system, biology, Macrophages, Solid Phase Extraction, 010401 analytical chemistry, Meth, 0104 chemical sciences, Cell biology, chemistry, biology.protein, Homeostasis, Chromatography, Liquid, medicine.drug

Abstract

Macrophages comprise a major component of the human innate immune system that is involved in maintaining homeostasis and responding to infections or other insults. Besides cytokines and chemokines, macrophages presumably influence the surrounding environment by secreting various types of metabolites. Characterization of secreted metabolites under normal and pathological conditions is critical for understanding the complex innate immune system. To investigate the secreted metabolome, we developed a novel workflow consisting of one Reverse Phase (RP) C18 column linked in tandem with a Cogent cholesterol-modified RP C18. This system was used to compare the secreted metabolomes of human monocyte-derived macrophages (hMDM) under normal conditions to those exposed to methamphetamine (Meth). This new experimental approach allowed us to measure 92 metabolites, identify 11 of them as differentially expressed, separate and identify three hydroxymethamphetamine (OHMA) isomers, and identify a new, yet unknown metabolite with a m/z of 192. This study is the first of its kind to address the secreted metabolomic response of hMDM to an insult by Meth. Besides the discovery of novel metabolites secreted by macrophages, we provide a novel methodology to investigate metabolomic profiling.

Published

2019

21. Improved Polycyclic Aromatic Hydrocarbon and n-Alkane Determination in Speleothems through Cleanroom Sample Processing

Author

Carlo Barbante, Elena Argiriadis, and Rhawn F. Denniston

Subjects

Liquid-Liquid Extraction, Sample processing, Polycyclic aromatic hydrocarbon, 010402 general chemistry, 01 natural sciences, Gas Chromatography-Mass Spectrometry, Analytical Chemistry, Limit of Detection, Cleanroom, Liquid–liquid extraction, Alkanes, Settore CHIM/01 - Chimica Analitica, Settore CHIM/12 - Chimica dell'Ambiente e dei Beni Culturali, Alkane, chemistry.chemical_classification, Detection limit, speleothems, 010401 analytical chemistry, Australia, Polycyclic aromatic hydrocarbons, Polycyclic aromatic hydrocarbons, n-alkanes, stalagmites, speleothems, cleanroom, 0104 chemical sciences, Molecular Weight, Caves, Italy, cleanroom, chemistry, Settore GEO/08 - Geochimica e Vulcanologia, Environmental chemistry, Environmental Pollutants, n-alkanes, stalagmites

Abstract

Interest in paleoenvironmental reconstructions from biomarkers in speleothems is increasing, thanks in part to the capacity of speleothems to grow continuously and to resist postdepositional alteration. In particular, the possibility exists to link high-resolution and accurately dated fire and vegetation records with isotopic data of climatic and paleoenvironmental interactions at the local and regional scale. However, the scarcity of existing methods for the quantification of organic molecules in stalagmites, together with the issues of sample availability, contamination, and low concentrations, complicate this approach. In this work, we developed a novel method for the simultaneous determination of 18 polycyclic aromatic hydrocarbons (PAHs) and 26 n-alkanes (C

Published

2019

22. Electrochemically Modulated Liquid–Liquid Extraction for Sample Enrichment

Author

Bahruddin Saad, Afidah Abdul Rahim, Marc Hébrant, Grégoire Herzog, Maizatul Najwa Jajuli, M. Hazwan Hussin, Universiti Sains Malaysia (USM), Laboratoire de Chimie Physique et Microbiologie pour les Matériaux et l'Environnement (LCPME), and Institut de Chimie du CNRS (INC)-Université de Lorraine (UL)-Centre National de la Recherche Scientifique (CNRS)

Subjects

Phenyl biguanide, Chromatography, Aqueous solution, endocrine system diseases, Chemistry, Liquid-Liquid Extraction, 010401 analytical chemistry, Extraction (chemistry), Biguanides, Electrochemical Techniques, Phenformin, 010402 general chemistry, 01 natural sciences, Sample (graphics), Metformin, 0104 chemical sciences, Analytical Chemistry, Quaternary Ammonium Compounds, chemistry.chemical_compound, [CHIM.ANAL]Chemical Sciences/Analytical chemistry, Liquid–liquid extraction, Sample preparation, Hydrophobic and Hydrophilic Interactions, Chromatography, High Pressure Liquid

Abstract

International audience; A new sample preparation method is proposed for the extraction of pharmaceutical compounds (Metformin, Phenyl biguanide, and Phenformin) of varied hydrophilicity, dissolved in an aqueous sample. When in contact with an organic phase, an interfacial potential is imposed by the presence of an ion, tetramethylammonium (TMA +), common to each phase. The interfacial potential difference drives the transfer of ionic analytes across the interface and allows to reach up to nearly 100 % extraction efficiency and a 60-fold enrichment factor in optimised extraction conditions as it is determined by HPLC analysis. 2

Published

2019

23. Bioprofiling of Surface/Wastewater and Bioquantitation of Discovered Endocrine-Active Compounds by Streamlined Direct Bioautography.

Author

Klingelhöfer, Ines and Morlock, Gertrud E.

Subjects

*ESTROGEN, *XENOESTROGENS, *LIQUID-liquid extraction, *WATER research, *ANALYTICAL chemistry research

Abstract

A direct bioautography has been used for the simultaneous determination of four estrogens [estrone (E1), 17β-estradiol (E2), estriol (E3), and 17α-ethinylestradiol (EE2)] and two xenoestrogens [bisphenol A (BPA) and 4-n-nonyl-phenol (NP)] in surface water and wastewater samples from a sewage treatment plant. After either direct application or a liquid--liquid extraction of the water samples, the qualitative and quantitative detection of estrogen-effective compounds was performed with a planar yeast estrogen screen. The limits of detection were different for each compound, due to the specific receptor binding of individual (xeno)estrogens (1 ng/L to 15 μg/L). The mean recovery rate for all six substances at this ultratrace level was 88% [mean percent relative standard deviation (%RSD) of 17%, n = 3]. Over the whole procedure, precisions of three estrogens discovered in a wastewater sample were below 17%, n = 3. The identification of the detected bioactive compounds was performed by high-performance thin-layer chromatography--electrospray ionization mass spectrometry (HPTLC--ESI-MS) via the elution-head-based TLC--MS Interface. Whereas the estrogens E1 and E2 could always be detected in the influent of the treatment plant, E3 was detected occasionally. The concentrations of E1 and E2 ranged from 3 to 50 ng/L, and for E3 from 98 to 210 ng/L. EE2, BPA, and NP could not be detected at the given LOD. In every second surface water sample, E1 and E2 were detected, but not E3, EE2, BPA, and NP. [ABSTRACT FROM AUTHOR]

Published

2015

24. Real-Time Volumetric Phase Monitoring: Advancing Chemical Analysis by Countercurrent Separation.

Author

Pauli, Guido F., Pro, Samuel M., Chadwick, Lucas R., Burdick, Thomas, Pro, Luke, Friedl, Warren, Novak, Nick, Maltby, John, Feng Qiu, and Brent Friesen, J.

Subjects

*COUNTERCURRENT processes, *PHASE separation, *LIQUID-liquid extraction, *REAL-time control, *AUTOMATIC control systems, *ANALYTICAL chemistry

Abstract

Countercurrent separation (CCS) utilizes the differential partitioning behavior of analytes between two immiscible liquid phases. We introduce the first platform ("CherryOne") capable of real-time monitoring, metering, and control of the dynamic liquid-liquid CCS process. Automated phase monitoring and volumetrics are made possible with an array of sensors, including the new permittivity-based phase metering apparatus (PMA). Volumetric data for each liquid phase are converted into a dynamic real-time display of stationary phase retention (Sf) and eluent partition coefficients (K), which represent critical parameters of CCS reproducibility. When coupled with the elution-extrusion operational mode (EECCC), automated Sf and K determination empowers untargeted and targeted applications ranging from metabolomic analysis to preparative purifications. [ABSTRACT FROM AUTHOR]

Published

2015

25. A Microfluidic Platform for the Rapid Determination of Distribution Coefficients by Gravity-Assisted Droplet-Based Liquid-Liquid Extraction.

Author

Poulsen, Carl Esben, Wootton, Robert C. R., Wolff, Anders, deMello, Andrew J., and Elvira, Katherine S.

Subjects

*MICROFLUIDICS, *LIQUID-liquid extraction, *PHASE separation, *CLINICAL drug trials, *DISSOCIATION (Chemistry)

Abstract

The determination of pharmacokinetic properties of drugs, such as the distribution coefficient (D) is a crucial measurement in pharmaceutical research. Surprisingly, the conventional (gold standard) technique used for D measurements, the shake-flask method, is antiquated and unsuitable for the testing of valuable and scarce drug candidates. Herein, we present a simple microfluidic platform for the determination of distribution coefficients using droplet-based liquid-liquid extraction. For simplicity, this platform makes use of gravity to enable phase separation for analysis and is 48 times faster and uses 99% less reagents than performing an equivalent measurement using the shake-flask method. Furthermore, the D measurements achieved in our platform are in good agreement with literature values measured using traditional shake-flask techniques. Since D is affected by volume ratios, we use the apparent acid dissociation constant, pK', as a proxy for intersystem comparison. Our platform determines a pK' value of 7.24 ± 0.15, compared to 7.25 ± 0.58 for the shake-flask method in our hands and 7.21 for the shake-flask method in the literature. Devices are fabricated using injection molding, the batchwise fabrication time is <2 min per device (at a cost of $1 U.S. per device), and the interdevice reproducibility is high. [ABSTRACT FROM AUTHOR]

Published

2015

26. Quantification of Nerve Agent Biomarkers in Human Serum and Urine.

Author

Røen, Bent Tore, Sellevåg, Stig Rune, and Lundanes, Elsa

Subjects

*BIOMARKERS, *SERUM, *URINE, *METABOLITES, *LIQUID-liquid extraction, *SOLID phase extraction

Abstract

A novel method for rapid and sensitive quantification of the nerve agent metabolites ethyl, isopropyl, isobutyl, cyclohexyl, and pinacolyl methylphosphonic acid has been established by combining salting-out assisted liquid-liquid extraction (SALLE) and online solid phase extraction-liquid chromatography-tandem mass spectrometry (SPE-LC-MS/MS). The procedure allows confirmation of nerve agent exposure within 30 min from receiving a sample, with very low detection limits for the biomarkers of 0.04-0.12 ng/mL. Sample preparation by SALLE was performed in less than 10 min, with a common procedure for both serum and urine. Analyte recoveries of 70-100% were obtained using tetrahydrofuran as extraction solvent and Na2SO4 to achieve phase separation. After SALLE, selective analyte retention was obtained on a ZrO2 column by Lewis acid-base and hydrophilic interactions with acetonitrile/1% CH3COOH (82/18) as the loading mobile phase. The phosphonic acids were backflush-desorbed onto a polymeric zwitterionic column at pH 9.8 and separated by hydrophilic interaction liquid chromatography. The method was linear (R2 ⩾ 0.995) from the limits of quantification to 50 ng/mL, and the within- and between-assay repeatability at 20 ng/mL were below 5% and 10% relative standard deviation, respectively. [ABSTRACT FROM AUTHOR]

Published

2014

27. Separation of Glycolipids/Sphingolipids from Glycerophospholipids on TiO

Author

Zehui, Huang, Qian, Wu, Hongmei, Lu, Yang, Wang, and Zhimin, Zhang

Subjects

Titanium, Sphingolipids, Limit of Detection, Lipidomics, Liquid-Liquid Extraction, Animals, Humans, Adsorption, Glycerophospholipids, Glycolipids, Mass Spectrometry, Rats

Abstract

In lipidomic analysis by direct mass spectrometry (MS), high abundance lipids with high ionizability (such as glycerophospholipids) would cause ion suppression to lipids with poor ionizability and low abundance (such as glycolipids, sphingolipids, or glycerides), which largely limits the detection coverage for lipidomics. In this work, TiO

Published

2020

28. LESA Cyclic Ion Mobility Mass Spectrometry of Intact Proteins from Thin Tissue Sections

Author

Emma K. Sisley, Helen J. Cooper, Kevin Giles, Francisco Fernandez-Lima, Martin Palmer, and Jakub Ujma

Subjects

Ion-mobility spectrometry, Surface Properties, Liquid-Liquid Extraction, 010402 general chemistry, Mass spectrometry, Kidney, 01 natural sciences, Article, Analytical Chemistry, Ion, Hemoglobins, Mice, Ion Mobility Spectrometry, Animals, Range (particle radiation), Chromatography, Chemistry, 010401 analytical chemistry, Extraction (chemistry), Brain, Proteins, 0104 chemical sciences, Rats, Tissue sections, Mass spectrum, One pass

Abstract

Liquid extraction surface analysis (LESA) is an ambient surface sampling technique that allows the analysis of intact proteins directly from tissue samples via mass spectrometry. Integration of ion mobility separation to LESA mass spectrometry workflows has shown significant improvements in the signal-to-noise ratios of the resulting protein mass spectra and hence the number of proteins detected. Here, we report the use of a quadrupole-cyclic ion mobility-time-of-flight mass spectrometer (Q-cIM-ToF) for the analysis of proteins from mouse brain and rat kidney tissues sampled via LESA. Among other features, the instrument allows multiple pass cyclic ion mobility separation, with concomitant increase in resolving power. Single-pass experiments enabled the detection of 30 proteins from mouse brain tissue, rising to 44 when quadrupole isolation was employed. In the absence of ion mobility separation, 21 proteins were detected in rat kidney tissue including the abundant α- and β-globin chains from hemoglobin. Single-pass cyclic ion mobility mass spectrometry enabled the detection of 60 additional proteins. Multipass experiments of a narrow m/z range (m/z 870-920) resulted in the detection of 24 proteins (one pass), 37 proteins (two passes) and 54 proteins (three passes), thus demonstrating the benefits of improved mobility resolving power.

Published

2020

29. High-Throughput Liquid-Liquid Extractions with Nanoliter Volumes

Author

Shane S. Wells and Robert T. Kennedy

Subjects

Detection limit, Electrospray, Analyte, Chromatography, Capillary action, 010401 analytical chemistry, Extraction (chemistry), Liquid-Liquid Extraction, Ethyl acetate, 010402 general chemistry, Mass spectrometry, 01 natural sciences, Article, 0104 chemical sciences, Analytical Chemistry, Partition coefficient, chemistry.chemical_compound, chemistry, Pharmaceutical Preparations, Limit of Detection, Calibration, Humans

Abstract

Liquid-liquid extractions are an important tool in chemistry. They are low cost and provide easy method development for purification, sample clean-up for analysis, and determination of physical constants such as partition coefficient. Current methods for liquid-liquid extractions generally require microliter to milliliter volumes of solvents and sample, long equilibration times, and manual procedures. Extraction methods for samples in microfluidic systems have been limited as this tool is difficult to implement on the nanoliter or smaller scale. We have developed slug-flow nanoextraction (SFNE), a method based on droplet microfluidics that allows multiple liquid-liquid extractions to be performed simultaneously in a capillary tube, using only 5 nL sample and extraction solvent per extraction. SFNE is performed by flowing adjacent plugs of extraction phase and aqueous (sample) phase (known as phase pairs or two-phase slugs) through a conduit. Recirculation within droplets during flow facilitates extraction across the phase pair interface. Each two-phase slug is segmented from the others by immiscible carrier fluid, in this case pefluorodecalin. In characterizing SFNE using a fluorescent dye, we found rapid extractions (< 5 s), partition coefficients that matched those achieved at larger scale extractions, and potential to preconcentrate samples through manipulation of the sample and extraction volume phase ratio. We coupled SFNE to on-line UV absorbance detection so that concentration of analytes can determined in each phase. This method was used to accurately and rapidly determine octanol-water partition coefficients (K(ow)). The K(ow) determined for acetaminophen by SFNE matched the value determined by the shake-flask method in the experiment at K(ow) = 2.48 ± 0.02. The measurement, along with calibration and 12 replicates, was complete within 5 min while consuming under 150 nL of solvent and sample. The method was also applied to extract analytes from complex biological samples prior to electrospray ionization-mass spectrometry (ESI-MS). A tube filled with two-phase slugs was pumped into an ESI source at 0.5 μL/min, corresponding to 6 s per sample. SFNE coupled to ESI-MS/MS was applied for simultaneous determination of five different drugs spiked into human plasma, synthetic urine (SU), and artificial cerebral spinal fluid (aCSF) using ethyl acetate as the extraction phase. The signal-to-noise (S/N) for analytes measured by mass spectrometry improved up to19-fold compared to direct ESI-MS of single-phase droplets (aqueous plugs segmented by carrier fluid), with limits of detection down to 7 nM (35 amol). The improved S/N is attributed to reduction of ionization suppression from the complex matrix by extraction of analyte into the organic phase.

Published

2020

30. LESA MS Imaging of Heat-Preserved and Frozen Tissue: Benefits of Multistep Static FAIMS

Author

Richard J. A. Goodwin, Anna L. Simmonds, Helen J. Cooper, Rian L. Griffiths, and John G. Swales

Subjects

Male, 0301 basic medicine, Hot Temperature, Surface Properties, Ion-mobility spectrometry, Liquid-Liquid Extraction, Single step, Kidney, Mass spectrometry, 01 natural sciences, Mass spectrometry imaging, Analytical Chemistry, 03 medical and health sciences, Tandem Mass Spectrometry, Ion Mobility Spectrometry, Testis, Animals, Rats, Wistar, Frozen tissue, Brain Chemistry, Chromatography, Chemistry, 010401 analytical chemistry, Proteins, 0104 chemical sciences, Cold Temperature, 030104 developmental biology, Tissue sections, High field, Asymmetric waveform

Abstract

We have previously demonstrated liquid extraction surface analysis (LESA) high field asymmetric waveform ion mobility spectrometry (FAIMS) mass spectrometry imaging of proteins in thin tissue sections of brain and liver. Here, we present an improved approach that makes use of multiple static FAIMS parameters at each sampled location and allows a significant improvement in the number of proteins, lipids, and drugs that can be imaged simultaneously. The approach is applied to the mass spectrometry imaging of control and cassette-dosed rat kidneys. Mass spectrometry imaging of kidneys typically requires washing to remove excess hemoglobin; however, that is not necessary with this approach. Multistep static FAIMS mass spectrometry resulted in a 6- to 16-fold increase in the number of proteins detected in the absence of FAIMS, in addition to smaller increases over single step static FAIMS (chosen for optimum transmission of total protein ions). The benefits of multistep static FAIMS mass spectrometry for protein detection are also shown for sections of testes. The numbers of proteins detected following multistep FAIMS increased between 2- and 3-fold over single step FAIMS and between 2- and 14-fold over LESA alone. Finally, to date, LESA mass spectrometry of proteins in tissue has been undertaken solely on fresh frozen samples. In this work, we demonstrate that heat-preserved tissues are also suitable for these analyses. Heat preservation of tissue improved the number of proteins detected by LESA MS for both kidney and testes tissue (by between 2- and 4-fold). For both tissue types, the majority of the proteins additionally detected in the heat-treated samples were subsequently detected in the frozen samples when FAIMS was incorporated. Improvements in the numbers of proteins detected were observed for LESA FAIMS MS for the kidney tissue; for testes tissue, fewer total proteins were detected following heat preservation; however, approximately one-third were unique to the heat-preserved samples.

Published

2018

31. In Vitro Liquid Extraction Surface Analysis Mass Spectrometry (ivLESA-MS) for Direct Metabolic Analysis of Adherent Cells in Culture

Author

Amanda R Clark, Nicholas D. Schmitt, Michael S. Regan, Jeffrey N. Agar, Nathalie Y. R. Agar, Sankha S. Basu, Elizabeth C. Randall, Begoña Gimenez-Cassina Lopez, and Deborah A. Dillon

Subjects

Spectrometry, Mass, Electrospray Ionization, Liquid-Liquid Extraction, Cell, Mass spectrometry, 01 natural sciences, Article, Analytical Chemistry, 03 medical and health sciences, 0302 clinical medicine, Metabolomics, Cell Line, Tumor, Monolayer, medicine, Humans, Nanotechnology, Sample preparation, Chromatography, High Pressure Liquid, Chromatography, Chemistry, 010401 analytical chemistry, Extraction (chemistry), Lipids, In vitro, Culture Media, 0104 chemical sciences, medicine.anatomical_structure, Cell culture, 030220 oncology & carcinogenesis

Abstract

Conventional metabolomic methods include extensive sample preparation steps and long analytical run times, increasing the likelihood of processing artifacts and limiting high throughput applications. We present here in vitro liquid extraction surface analysis mass spectrometry (ivLESA-MS), a variation on LESA-MS, performed directly on adherent cells grown in 96-well cell culture plates. To accomplish this, culture medium was aspirated immediately prior to analysis, and metabolites were extracted using LESA from the cell monolayer surface, followed by nano-electrospray ionization and MS analysis in negative ion mode. We applied this platform to characterize and compare lipidomic profiles of multiple breast cancer cell lines growing in culture (MCF-7, ZR-75–1, MDA-MB-453, and MDA-MB-231) and revealed distinct and reproducible lipidomic signatures between the cell lines. Additionally, we demonstrated time-dependent processing artifacts, underscoring the importance of immediate analysis. ivLESA-MS represents a rapid in vitro metabolomic method, which precludes the need for quenching, cell harvesting, sample preparation, and chromatography, significantly shortening preparation and analysis time while minimizing processing artifacts. This method could be further adapted to test drugs in vitro in a high throughput manner.

Published

2018

32. Microfluidic Droplet-Based Liquid–Liquid Extraction and On-Chip IR Spectroscopy Detection of Cocaine in Human Saliva.

Author

Wägli, Philip, Yu-Chi Chang, Homsy, Alexandra, Hvozdara, Lubos, Herzig, Hans Peter, and de Rooij, Nico F.

Subjects

*MICROFLUIDIC analytical techniques, *INFRARED spectroscopy techniques, *COCAINE, *SALIVA analysis, *LIQUID-liquid extraction

Abstract

We present a portable microsystem to quantitatively detect cocaine in human saliva. In this system, we combine a microfluidic-based multiphase liquid-liquid extraction method to transfer cocaine continuously from IR-light-absorbing saliva to an IR-transparent solvent (tetrachloroethylene) with waveguide IR spectroscopy (QC-laser, waveguide, detector) to detect the cocaine on-chip. For the fabrication of the low-cost polymer microfluidic chips a simple rapid prototyping technique based on Scotch-tape masters was further developed and applied. To perform the droplet-based liquid-liquid extraction, we designed and integrated a simple and robust droplet generation method based on the capillary focusing effect within the device. Compared to well-characterized and commonly used microfluidic H-filters, our system showed at least two times higher extraction efficiencies with potential for further improvements. The current liquid-liquid extraction method alone can efficiently extract cocaine and pre-concentrate the analytes in a new solvent. Our fully integrated optofluidic system successfully detected cocaine in real saliva samples spiked with the drug (500 μg/mL) and allowed real time measurements, which makes this approach suitable for point-of-care applications. [ABSTRACT FROM AUTHOR]

Published

2013

33. Ultra Performance Liquid Chromatography-Tandem Mass Spectrometry Method for Profiling of Steroid Metabolome in Human Tissue.

Author

Gaikwad, Nilesh W.

Subjects

*HIGH performance liquid chromatography, *TANDEM mass spectrometry, *TISSUE analysis, *METABOLITE analysis, *STEROID metabolism, *LIQUID-liquid extraction, *STEROID hormones, *ESTROGEN

Abstract

In humans, steroids play a broad and vital role in regulation of gene expression, secondary sexual characteristics, maturation, reproduction, cardiovascular health, neurological functions, etc., but imbalance in steroid metabolism is also linked to development and progression of many diseases, such as cancer, neurodegenerative diseases, and cardiovascular diseases. Hence, measurement of steroids in biological samples is essential to monitor human health. Currently, there is radioimmunoassay, gas chromatography-mass spectrometry (GC/MS), and liquid chromatography–mass spectrometry (LC-MS) methods developed for steroid measurements in biological samples. However, these methods require elaborate sample preparation procedures and have concerns(s) related to reproducibility, dynamic range, time, costs, and most importantly the total coverage of steroids. Also currently, there is no method available for comprehensive steroid profiling in a single LC-MS run that includes androgens, corticosteroids, progestogens, estrogens, estrogen metabolites, estrogen conjugates, and estrogen-DNA adducts as well as exogenous steroid derivatives. Here, I present a global steroid metabolic profiling method based on liquid–liquid extraction (LLE) followed by ultra performance liquid chromatography (UPLC)-tandem mass spectrometry (MS/MS) for simultaneous measurement of over 100 indigenous as well as exogenous steroids in about 12 min, without derivatization. The method was successfully applied to determine steroid hormone levels in the breast tissue of healthy women. Overall presence of all major classes of steroids as well as estrogen derivatives was detected in breast tissue. [ABSTRACT FROM AUTHOR]

Published

2013

34. Automated Liquid-Liquid Extraction by Pneumatic Recirculation on a Centrifugal Microfluidic Platform.

Author

Kazarine, Alexei, Kong, Matthew C. R., Templeton, Erin J., and Salin, Eric D.

Subjects

*LIQUID-liquid extraction, *EXTRACTION techniques, *MICROFLUIDIC devices, *MICROFLUIDIC analytical techniques, *AUTOMATION, *PNEUMATICS, *CHEMICAL sample preparation

Abstract

In this technical note, a liquid–liquid extraction technique was performed using pneumatic liquid recirculation on a centrifugal microfluidic device. Non-contact pneumatic pumping enabled a multi-cycle liquid–liquid extraction process using aqueous iodine in a potassium iodide solution and hexadecane while requiring a minimal amount of space on the device. The extraction process was completely automated on the device following sample introduction and required only 50 s for each extraction cycle. The pumping rate achieved during liquid recirculation was 120 ± 10 μL/min. A recycling process such as the one demonstrated would be difficult to implement in a conventional centrifugal microfluidic system. [ABSTRACT FROM AUTHOR]

Published

2012

35. Aerosol-Phase Extraction Method for Determination of Ca, K, Mg, and Na in Biodiesel through Inductively Coupled Plasma Optical Emission Spectrometry

Author

José-Luis Todolí, Salvador E. Maestre, Soledad Prats, Raquel Barragán Sánchez, Universidad de Alicante. Departamento de Química Analítica, Nutrición y Bromatología, Análisis de Polímeros y Nanomateriales, and Análisis de Alimentos y Nutrición

Subjects

Aerosol phase extraction, Analytical chemistry, Liquid – liquid Extraction, 02 engineering and technology, 01 natural sciences, Analytical Chemistry, chemistry.chemical_compound, Nitric acid, Liquid–liquid extraction, Aqueous solution, Chromatography, 010401 analytical chemistry, Extraction (chemistry), Aqueous two-phase system, 021001 nanoscience & nanotechnology, Nutrición y Bromatología, 0104 chemical sciences, chemistry, Metals, Elemental analysis, Inductively coupled plasma atomic emission spectroscopy, ICP-OES, Química Analítica, Biodiesel, Inductively coupled plasma, 0210 nano-technology

Abstract

A novel extraction method was developed, optimized, and validated for the elemental analysis of organic samples. The method, called aerosol-phase extraction (APE), is based on nebulization of the extracting aqueous solution (0.1 mol·L–1 nitric acid) on the sample. Extraction was performed at the interface of generated extractant droplets as they entered into contact with the samples. Afterward, the phases were allowed to separate and Ca, K, Na, and Mg were determined in aqueous phase by means of inductively coupled plasma optical emission spectroscopy (ICP-OES). Measurement of aerosol characteristics demonstrated that a water-in-oil emulsion was generated. Therefore, once the aqueous solution was dispersed into the sample, the phases spontaneously separated. Furthermore, the interfacial specific surface area exhibited values on the order of 1 m2·mL–1, hence enhancing the extraction kinetics over conventional extraction methods. Key variables affecting the extraction yield were the nebulization gas flow rate, liquid flow rate, extraction time, acid concentration, nebulizer tip to sample surface gap, and morg/maq ratio. Once the optimal conditions were selected, the method was applied and validated for the determination of Ca, K, Na, and Mg by ICP-OES in 0.5 mL biodiesel samples with an expanded uncertainty lower than 2%. With the APE method, the extraction time was around 1 min, whereas conventional methods employed to perform this kind of extraction required from 4 to 50 min. Additionally, the APE involved preconcentration of analytes, thus lowering the limit of detection (LOD) to the nanograms per milliliter level (i.e., LODs based on the 3sb criterion were 32, 20, 19, and 24 ng·mL–1 for Ca, K, Na, and Mg, respectively). Furthermore, accuracy of quantification of Ca, K, Na, and Mg concentration by APE was not significantly different as compared to that afforded by conventional liquid–liquid extraction. Finally, Ca, K, Na, and Mg contents were determined in four real samples in the 0.5–13 mg·kg–1 range. The obtained results were not statistically different from those encountered with a microwave-based digestion method.

Published

2017

36. FAST: Size-Selective, Clog-Free Isolation of Rare Cancer Cells from Whole Blood at a Liquid–Liquid Interface

Author

Hyeongeun Kim, Hyunjin Jeong, Juhee Park, Gwang Ha Kim, Sungmok Jung, Minji Lim, Jung Min Oh, Byung Chul Kim, Yoon-Kyoung Cho, Hee Chul Park, Sun Ju Lee, Mi-Hyun Kim, Do Youn Park, Kyu-Sang Lee, and Tae-Hyeong Kim

Subjects

0301 basic medicine, Time Factors, Isolation (health care), Liquid-Liquid Extraction, Nanotechnology, Cell Separation, Analytical Chemistry, 03 medical and health sciences, 0302 clinical medicine, Circulating tumor cell, Cell Line, Tumor, Neoplasms, medicine, Humans, Liquid liquid, General hospital, Cell Size, Whole blood, Chemistry, Cancer, Equipment Design, Microfluidic Analytical Techniques, Neoplastic Cells, Circulating, medicine.disease, Rare cancer, 030104 developmental biology, 030220 oncology & carcinogenesis, Size selective, Biomedical engineering

Abstract

Circulating tumor cells (CTCs) have great potential to provide minimally invasive ways for the early detection of cancer metastasis and for the response monitoring of various cancer treatments. Despite the clinical importance and progress of CTC-based cancer diagnostics, most of the current methods of enriching CTCs are difficult to implement in general hospital settings due to complex and time-consuming protocols. Among existing technologies, size-based isolation methods provide antibody-independent, relatively simple, and high throughput protocols. However, the clogging issues and lower than desired recovery rates and purity are the key challenges. In this work, inspired by antifouling membranes with liquid-filled pores in nature, clog-free, highly sensitive (95.9 ± 3.1% recovery rate), selective (2.5 log depletion of white blood cells), rapid (3 mL/min), and label-free isolation of viable CTCs from whole blood without prior sample treatment is achieved using a stand-alone lab-on-a-disc system equipped with fluid-assisted separation technology (FAST). Numerical simulation and experiments show that this method provides uniform, clog-free, ultrafast cell enrichment with pressure drops much less than in conventional size-based filtration, at 1 kPa. We demonstrate the clinical utility of the point-of-care detection of CTCs with samples taken from 142 patients suffering from breast, stomach, or lung cancer.

Published

2016

37. Quantitative Imaging of Proteins in Tissue by Stable Isotope Labeled Mimetic Liquid Extraction Surface Analysis Mass Spectrometry

Author

Elizabeth C. Randall, John G. Swales, Iain B. Styles, Rian L. Griffiths, Helen J. Cooper, Richard J. A. Goodwin, Josephine Bunch, and Jana Havlikova

Subjects

Quantitative imaging, Letter, Liquid-Liquid Extraction, Endogeny, 010402 general chemistry, Mass spectrometry, 01 natural sciences, Mass Spectrometry, Analytical Chemistry, Mice, Ubiquitin, Animals, Sample preparation, Brain Chemistry, Chromatography, biology, Stable isotope ratio, Chemistry, Spatially resolved, 010401 analytical chemistry, 0104 chemical sciences, Rats, biology.protein, Homogenization (biology), Chromatography, Liquid

Abstract

Absolute quantification of proteins in tissue is important for numerous fields of study. Liquid chromatography–mass spectrometry (LC–MS) methods are the norm but typically involve lengthy sample preparation including tissue homogenization, which results in the loss of information relating to spatial distribution. Here, we propose liquid extraction surface analysis (LESA) mass spectrometry (MS) of stable isotope labeled mimetic tissue models for the spatially resolved quantification of intact ubiquitin in rat and mouse brain tissue. Measured ubiquitin concentrations are in agreement with values found in the literature. Images of rat and mouse brain tissue demonstrate spatial variation in the concentration of ubiquitin and demonstrate the utility of spatially resolved quantitative measurement of proteins in tissue. Although we have focused on ubiquitin, the method has the potential for broader application to the absolute quantitation of any endogenous protein or protein-based drug in tissue.

Published

2019

38. Direct Depolymerization Coupled to Liquid Extraction Surface Analysis-High-Resolution Mass Spectrometry for the Characterization of the Surface of Plant Tissues

Author

Edwige Moyroud, Markus Kalberer, Chiara Giorio, Beverley J. Glover, Giorio, Chiara [0000-0001-7821-7398], and Apollo - University of Cambridge Repository

Subjects

Chromatography, Chemistry, Depolymerization, 010401 analytical chemistry, Extraction (chemistry), fungi, Liquid-Liquid Extraction, food and beverages, Flowers, 010402 general chemistry, 01 natural sciences, Mass Spectrometry, 0104 chemical sciences, Analytical Chemistry, Characterization (materials science), Plant Epidermis, Polymerization, Membrane Lipids, Epidermis (zoology), Hibiscus, Layer (electronics), Cuticle (hair)

Abstract

[Image: see text] The cuticle, the outermost layer covering the epidermis of most aerial organs of land plants, can have a heterogeneous composition even on the surface of the same organ. The main cuticle component is the polymer cutin which, depending on its chemical composition and structure, can have different biophysical properties. In this study, we introduce a new on-surface depolymerization method coupled to liquid extraction surface analysis (LESA) high-resolution mass spectrometry (HRMS) for a fast and spatially resolved chemical characterization of the cuticle of plant tissues. The method is composed of an on-surface saponification, followed by extraction with LESA using a chloroform–acetonitrile–water (49:49:2) mixture and direct HRMS detection. The method is also compared with LESA-HRMS without prior depolymerization for the analysis of the surface of the petals of Hibiscus richardsonii flowers, which have a ridged cuticle in the proximal region and a smooth cuticle in the distal region. We found that on-surface saponification is effective enough to depolymerize the cutin into its monomeric constituents thus allowing detection of compounds that were not otherwise accessible without a depolymerization step. The effect of the depolymerization procedure was more pronounced for the ridged/proximal cuticle, which is thicker and richer in epicuticular waxes compared with the cuticle in the smooth/distal region of the petal.

Published

2019

39. Ambient Ionization Mass Spectrometry: Recent Developments and Applications

Author

Rachel J. DeHoog, Clara L. Feider, Livia S. Eberlin, and Anna Krieger

Subjects

Diagnostic Imaging, Spectrometry, Mass, Electrospray Ionization, Bacteria, Extramural, Chemistry, Lasers, Liquid-Liquid Extraction, Analytical chemistry, Plants, Mass spectrometry, Article, Analytical Chemistry, Animals, Humans, Drug Monitoring, Organic Chemicals, Ambient ionization

Published

2019

40. Cloud-Point Extraction Combined with Thermal Degradation for Nanoplastic Analysis Using Pyrolysis Gas Chromatography-Mass Spectrometry

Author

Xiaoxia Zhou, Huang-ying-zi Wang, Li-teng Hao, Jingfu Liu, and Ying-jie Li

Subjects

Microplastics, Octoxynol, Liquid-Liquid Extraction, Glucuronates, Wastewater, 010402 general chemistry, Mass spectrometry, Disaccharides, 01 natural sciences, Analytical Chemistry, Surface-Active Agents, Rivers, Limit of Detection, Polymethyl Methacrylate, Seawater, Cloud point, Chromatography, Chemistry, 010401 analytical chemistry, Extraction (chemistry), Reproducibility of Results, Contamination, 0104 chemical sciences, Pyrolysis–gas chromatography–mass spectrometry, Nanoparticles, Polystyrenes, Enrichment factor, Pyrolysis, Water Pollutants, Chemical

Abstract

The contamination of micro- and nanoplastics in marine systems and freshwater is a global issue. Determination of micro- and nanoplastics in the aqueous environment is of high priority to fully assess the risk that plastic particles will pose. Although microplastics have been detected in a variety of aquatic ecosystems, the analysis of nanoplastics remains an unsolved challenge. Herein, for the first time, a Triton X-45 (TX-45)-based cloud-point extraction (CPE) was proposed to preconcentrate trace nanoplastics in environmental waters. Under the optimum extraction conditions, an enrichment factor of 500 was obtained for two types of nanoplastics with different compositions, polystyrene (PS) and poly(methyl methacrylate) (PMMA), without disturbing their original morphology and sizes. Additionally, following thermal treatment at 190 °C for 3 h, the CPE-obtained extract could be submitted to pyrolysis gas chromatography-mass spectrometry (Py-GC/MS) analysis for mass quantification of nanoplastics. Taking 66.2 nm PS nanoplastics and 86.2 nm PMMA nanoplastics as examples, the proposed method showed excellent reproducibility, and high sensitivity with respective detection limits of 11.5 and 2.5 fM. Feasibility of the proposed approach was verified by application of the optimized procedure to four real water samples. Recoveries of 84.6-96.6% at a spiked level of 88.6 fM for PS nanoplastics and 76.5-96.6% at a spiked level of 50.4 fM for PMMA nanoplastics were obtained. Consequently, this work provides an efficient approach for nanoplastic analysis in environmental waters.

Published

2018

41. Generic Enrichment of Organic Contaminants in Human Biomonitoring: Application in Monitoring Early Life Exposures to Fipronil via Breast Milk.

Author

Liu Z, Chen D, Lyu B, Li J, Zhao Y, and Wu Y

Subjects

Female, Humans, Liquid-Liquid Extraction, Pyrazoles, Biological Monitoring, Milk, Human

Abstract

In human biomonitoring, a high-throughput extraction and enrichment method for multiple types of organic contaminants at the part-per-trillion level is critical yet challenging, especially in the limited sample volume. When large-scale sample analysis is involved, low cost is often what we should consider. We describe a generic and straightforward cold-induced liquid-liquid extraction (CI-LLE) strategy to meet this need. Current methods for extracting and enriching organic contaminants from biological samples often require multistep sample processing, including specially tailoring the extraction solvent or adsorbents. This method uses cold-induced phase separation to achieve the extraction and enrichment of studied organic contaminants by adjusting the proportion of acetonitrile/water mixture, so as to integrate the extraction and enrichment in one step without additional reagents and adsorbents. In this study, fipronil insecticide was used as a representative compound to determine the key parameters of CI-LLE. The optimized CI-LLE procedure allowed simultaneous extraction and enrichment of studied organic contaminants, providing excellent enrichment factors (especially for lipophilic organic contaminants). CI-LLE was further applied in monitoring early life exposures of fipronil in 109 breast milk samples. This study provided baseline data on fipronil levels in breast milk samples from China. For infants, exposure to fipronil is of concern. In summary, CI-LLE provides a feasible solution for a generic, efficient, and low-cost preparation of biological samples and promotes high-throughput batch analysis of organic contaminants for large-scale human biomonitoring.

Published

2022

42. Sample Preparation for Bioanalytical and Pharmaceutical Analysis

Author

Cheng Zhang, Kevin D. Clark, and Jared L. Anderson

Subjects

Bioanalysis, Drug Industry, 010405 organic chemistry, Chemistry, Liquid-Liquid Extraction, Solid Phase Extraction, 010401 analytical chemistry, Protein Data Bank (RCSB PDB), Nanotechnology, DNA, Computational biology, 01 natural sciences, Biological Science Disciplines, Specimen Handling, 0104 chemical sciences, Analytical Chemistry, Pharmaceutical Preparations, RNA analysis, Animals, Humans, RNA, Sample preparation, Drug industry

Abstract

Biological and pharmaceutical samples represent formidable challenges in sample preparation that hold important consequences for bioanalysis and genotoxic impurity quantification. This Feature will emphasize significant advances toward the development of rapid, sensitive, and selective sample preparation methods.

Published

2016

43. Improved Extraction Repeatability and Spectral Reproducibility for Liquid Extraction Surface Analysis-Mass Spectrometry Using Superhydrophobic-Superhydrophilic Patterning

Author

Joris, Meurs, Morgan R, Alexander, Pavel A, Levkin, Simon, Widmaier, Josephine, Bunch, David A, Barrett, and Dong-Hyun, Kim

Subjects

Male, Vitamin B 12, Diphenhydramine, Raffinose, Rhodamines, Surface Properties, Taurine, Liquid-Liquid Extraction, Humans, Arginine, Hydrophobic and Hydrophilic Interactions, Healthy Volunteers, Mass Spectrometry

Abstract

A major problem limiting reproducible use of liquid extraction surface analysis (LESA) array sampling of dried surface-deposited liquid samples is the unwanted spread of extraction solvent beyond the dried sample limits, resulting in unreliable data. Here, we explore the use of the Droplet Microarray (DMA), which consists of an array of superhydrophilic spots bordered by a superhydrophobic material giving the potential to confine both the sample spot and the LESA extraction solvent in a defined area. We investigated the DMA method in comparison with a standard glass substrate using LESA analysis of a mixture of biologically relevant compounds with a wide mass range and different physicochemical properties. The optimized DMA method was subsequently applied to urine samples from a human intervention study. Relative standard deviations for the signal intensities were all reduced at least 3-fold when performing LESA-MS on the DMA surface compared with a standard glass surface. Principal component analysis revealed more tight clusters indicating improved spectral reproducibility for a human urine sample extracted from the DMA compared to glass. Lastly, in urine samples from an intervention study, more significant ions (145) were identified when using LESA-MS spectra of control and test urine extracted from the DMA. We demonstrate that DMA provides a surface-assisted LESA-MS method delivering significant improvement of the surface extraction repeatability leading to the acquisition of more robust and higher quality data. The DMA shows potential to be used for LESA-MS for controlled and reproducible surface extraction and for acquisition of high quality, qualitative data in a high-throughput manner.

Published

2018

44. Multielement Determination of Trace Heavy Metals in Water by Microwave-Induced Plasma Atomic Emission Spectrometry after Extraction in Unconventional Single-Salt Aqueous Biphasic System

Author

S. V. Smirnova, Dmitry Ilin, Tatiana O Samarina, and Igor V. Pletnev

Subjects

Detection limit, Cadmium, Aqueous solution, Metal ions in aqueous solution, Spectrophotometry, Atomic, 010401 analytical chemistry, Extraction (chemistry), Liquid-Liquid Extraction, chemistry.chemical_element, Water, 02 engineering and technology, Zinc, 021001 nanoscience & nanotechnology, 01 natural sciences, 0104 chemical sciences, Analytical Chemistry, chemistry, Reagent, Metals, Heavy, Salts, 0210 nano-technology, Microwaves, Cobalt, Water Pollutants, Chemical, Nuclear chemistry

Abstract

For the first time liquid–liquid extraction was used for the preconcentration of heavy metals prior to their determination in water by microwave-induced plasma atomic emission spectrometry (MP-AES). Extraction of Pb(II), Cd(II), Co(II), Ni(II), Zn(II), and Cu(II) was performed in unconventional aqueous biphasic system (ABS) formed by addition of hydrophobic solid salt, namely, tetrahexylammonium bromide, to aqueous sample, with neither organic solvents nor salting-out agents being used. The metal ions were quantitatively recovered with 4-(2-pyridylazo)-resorcinol (PAR). The extract was diluted with ethanol/HCl and introduced directly into an MP-AES instrument. The factors influencing extraction (pH, reagent concentration, phase contact time, etc.) and MP-AES detection parameters were studied and optimized. For the developed method, limits of detection of 1.3, 4.9, 0.06, 1.2, 4.2, and 3.2 μg L–1 were obtained for cadmium, cobalt, copper, nickel, lead, and zinc, respectively, providing from 60- to 500-fold ...

Published

2018

45. A Novel Approach for the Determination of the Ge Isotope Ratio Using Liquid-Liquid Extraction and Hydride Generation by Multicollector Inductively Coupled Plasma Mass Spectrometry.

Author

Karasiński J, Tupys A, Halicz L, and Bulska E

Subjects

Mass Spectrometry, Spectrum Analysis, Isotopes analysis, Liquid-Liquid Extraction

Abstract

In this work, a method for the accurate and precise determination of the Ge isotope ratio in synthetic water and natural samples of geological origin using multicollector inductively coupled plasma mass spectrometry (MC-ICPMS) with hydride generation was developed. The method was based on the liquid-liquid extraction of Ge to eliminate all elements affecting the generation of germanium hydrides. The standard-sample bracketing method was used to correct instrumental bias. Registration of analytical signal in time-resolved mode gave way to choose signals with best parameters and improved the precision of the results. Controlling the pH by using acetic buffer boosted the sensitivity by nearly five times in comparison to hydride generation methods suggested by other authors. The newly developed method is much simpler and quicker, does not need laborious Ge separation with ion-exchange resins, and thanks to its superior sensitivity, allows measurements of the Ge isotopic ratio in materials with relatively low Ge content. Delta values of the 74 Ge/ 70 Ge isotope ratio were measured in standard reference materials for which reference values were available in the GeoREM database. We demonstrated that the accuracy and precession of this method are equally good or better than methods proposed by other authors.

Published

2021

46. Ambient Mass Spectrometry Imaging Using Direct Liquid Extraction Techniques

Author

Ingela Lanekoff and Julia Laskin

Subjects

Analyte, Chromatography, Chemistry, Liquid-Liquid Extraction, 010401 analytical chemistry, Analytical technique, Analytical chemistry, 010402 general chemistry, Mass spectrometry, 01 natural sciences, Mass Spectrometry, Article, Mass spectrometry imaging, 0104 chemical sciences, Analytical Chemistry, Ionization, Animals, Humans, Sample preparation, Direct electron ionization liquid chromatography–mass spectrometry interface, Ambient ionization

Abstract

Mass spectrometry imaging (MSI) is a powerful analytical technique that enables label-free spatial localization and identification of molecules in complex samples.1-4 MSI applications range from forensics5 to clinical research6 and from understanding microbial communication7-8 to imaging biomolecules in tissues.1, 9-10 Recently, MSI protocols have been reviewed.11 Ambient ionization techniques enable direct analysis of complex samples under atmospheric pressure without special sample pretreatment.3, 12-16 In fact, in ambient ionization mass spectrometry, sample processing (e.g., extraction, dilution, preconcentration, or desorption) occurs during the analysis.17 This substantially speeds up analysis and eliminates any possible effects of sample preparation on the localization of molecules in the sample.3, 8, 12-14, 18-20 Venter and co-workers have classified ambient ionization techniques into three major categories based on the sample processing steps involved: 1) liquid extraction techniques, in which analyte molecules are removed from the sample and extracted into a solvent prior to ionization; 2) desorption techniques capable of generating free ions directly from substrates; and 3) desorption techniques that produce larger particles subsequently captured by an electrospray plume and ionized.17 This review focuses on localized analysis and ambient imaging of complex samples using a subset of ambient ionization methods broadly defined as “liquid extraction techniques” based onmore » the classification introduced by Venter and co-workers.17 Specifically, we include techniques where analyte molecules are desorbed from solid or liquid samples using charged droplet bombardment, liquid extraction, physisorption, chemisorption, mechanical force, laser ablation, or laser capture microdissection. Analyte extraction is followed by soft ionization that generates ions corresponding to intact species. Some of the key advantages of liquid extraction techniques include the ease of operation, ability to analyze samples in their native environments, speed of analysis, and ability to tune the extraction solvent composition to a problem at hand. For example, solvent composition may be optimized for efficient extraction of different classes of analytes from the sample or for quantification or online derivatization through reactive analysis. In this review, we will: 1) introduce individual liquid extraction techniques capable of localized analysis and imaging, 2) describe approaches for quantitative MSI experiments free of matrix effects, 3) discuss advantages of reactive analysis for MSI experiments, and 4) highlight selected applications (published between 2012 and 2015) that focus on imaging and spatial profiling of molecules in complex biological and environmental samples.« less

Published

2015

47. Cloud Point Extraction for Electroanalysis: Anodic Stripping Voltammetry of Cadmium

Author

William R. Heineman, Adam Bange, Cory A. Rusinek, and Ian Papautsky

Subjects

Cloud point, Stripping (chemistry), Octoxynol, Chemistry, Metal ions in aqueous solution, Liquid-Liquid Extraction, Inorganic chemistry, Extraction (chemistry), Analytical chemistry, Electrochemical Techniques, Iodides, Sulfuric Acids, Article, Polyethylene Glycols, Analytical Chemistry, Surface-Active Agents, Anodic stripping voltammetry, Liquid–liquid extraction, Electroanalytical method, Electrodes, Voltammetry, Water Pollutants, Chemical, Cadmium

Abstract

Cloud point extraction (CPE) is a well-established technique for the preconcentration of hydrophobic species from water without the use of organic solvents. Subsequent analysis is then typically performed via atomic absorption spectroscopy (AAS), UV-vis spectroscopy, or high performance liquid chromatography (HPLC). However, the suitability of CPE for electroanalytical methods such as stripping voltammetry has not been reported. We demonstrate the use of CPE for electroanalysis using the determination of cadmium (Cd(2+)) by anodic stripping voltammetry (ASV). Rather than using the chelating agents which are commonly used in CPE to form a hydrophobic, extractable metal complex, we used iodide and sulfuric acid to neutralize the charge on Cd(2+) to form an extractable ion pair. This offers good selectivity for Cd(2+) as no interferences were observed from other heavy metal ions. Triton X-114 was chosen as the surfactant for the extraction because its cloud point temperature is near room temperature (22-25 °C). Bare glassy carbon (GC), bismuth-coated glassy carbon (Bi-GC), and mercury-coated glassy carbon (Hg-GC) electrodes were compared for the CPE-ASV. A detection limit for Cd(2+) of 1.7 nM (0.2 ppb) was obtained with the Hg-GC electrode. ASV with CPE gave a 20x decrease (4.0 ppb) in the detection limit compared to ASV without CPE. The suitability of this procedure for the analysis of tap and river water samples was demonstrated. This simple, versatile, environmentally friendly, and cost-effective extraction method is potentially applicable to a wide variety of transition metals and organic compounds that are amenable to detection by electroanalytical methods.

Published

2015

48. Quantitative Spatial Analysis of the Mouse Brain Lipidome by Pressurized Liquid Extraction Surface Analysis

Author

Jan Baumgart, Zane Berzina, Reinaldo Almeida, Robert Nitsch, Eva C. Arnspang, Johannes Vogt, and Christer S. Ejsing

Subjects

Male, In situ, Chromatography, Chemistry, Liquid-Liquid Extraction, Extraction (chemistry), Analytical chemistry, Brain, Shotgun lipidomics, Lipidome, Mass spectrometry, Lipids, Mass Spectrometry, Fourier transform ion cyclotron resonance, Analytical Chemistry, Mice, Inbred C57BL, Mice, Microscopy, Fluorescence, Fragmentation (mass spectrometry), Liquid–liquid extraction, Spectroscopy, Fourier Transform Infrared, Pressure, Animals

Abstract

Here we describe a novel surface sampling technique termed pressurized liquid extraction surface analysis (PLESA), which in combination with a dedicated high-resolution shotgun lipidomics routine enables both quantification and in-depth structural characterization of molecular lipid species extracted directly from tissue sections. PLESA uses a sealed and pressurized sampling probe that enables the use of chloroform-containing extraction solvents for efficient in situ lipid microextraction with a spatial resolution of 400 μm. Quantification of lipid species is achieved by the inclusion of internal lipid standards in the extraction solvent. The analysis of lipid microextracts by nanoelectrospray ionization provides long-lasting ion spray which in conjunction with a hybrid ion trap-orbitrap mass spectrometer enables identification and quantification of molecular lipid species using a method with successive polarity shifting, high-resolution Fourier transform mass spectrometry (FTMS), and fragmentation analysis. We benchmarked the performance of the PLESA approach for in-depth lipidome analysis by comparing it to conventional lipid extraction of excised tissue homogenates and by mapping the spatial distribution and molar abundance of 170 molecular lipid species across different anatomical mouse brain regions.

Published

2015

49. Rapid Sample Preparation Using Slug Flow-Laminar Flow: Passive In Situ Microextraction/Stripping Coupling.

Author

Wang T, Wang W, Zheng Q, Ma Y, and Xu C

Subjects

Water, Liquid Phase Microextraction, Liquid-Liquid Extraction

Abstract

To increase the detection accuracy of radioactive samples, sample preparation through liquid-liquid extraction (LLE) before instrumental analysis is a crucial step. LLE preparation involves multiple steps including the tedious separation steps of co-extraction and stripping, which may cause sample loss, radioactive contamination, and radioactive leaks. In this study, a novel hybrid slug flow-laminar flow (SFLF) microchip in passive mode was designed to couple extraction and stripping in situ to realize a one-step sample preparation. The difficulty in maintaining stable water-organic-water interfaces was mitigated by using a partition wall and three resistance isolation areas. The mass transfer performance of the SFLF microchip was investigated and compared with that of the supported liquid membrane and three-layer laminar flow microextraction/stripping systems. Furthermore, the applicability of the SFLF system in preparing radioactive samples was validated through the selective separation of Ce and Pr from Cs and Sr. The novel SFLF microextraction/stripping system has a stable flow pattern, high mass transfer efficiency, and superior operating flexibility.

Published

2021

50. Liquid Extraction Surface Analysis Mass Spectrometry Method for Identifying the Presence and Severity of Nonalcoholic Fatty Liver Disease

Author

Zoe, Hall, Yajing, Chu, and Julian L, Griffin

Subjects

Diagnosis, Differential, Male, Mice, Liver, Non-alcoholic Fatty Liver Disease, Liquid-Liquid Extraction, Animals, Humans, Fatty Acids, Nonesterified, Mass Spectrometry, Triglycerides, Chromatography, Liquid

Abstract

The early stages of nonalcoholic fatty liver disease (NAFLD) are characterized by the accumulation of fat in the liver (steatosis). This can lead to cell injury and inflammation resulting in nonalcoholic steatohepatitis (NASH). To determine whether lipid profiling of liver tissue can identify metabolic signatures associated with disease presence and severity, we explored liquid extraction surface analysis mass spectrometry (LESA-MS) as a novel sampling tool. Using LESA-MS, lipids were extracted directly from the surface of ultrathin slices of liver tissue prior to detection by high-resolution mass spectrometry (MS). An isotopically labeled internal standard mix was incorporated into the extraction solvent to attain semiquantitative data. Data mining and multivariate statistics were employed to evaluate the generated lipid profiles and abundances. With this approach, we were able to differentiate healthy and NAFLD liver in mouse and human tissue samples, finding several triacylglyceride (TAG) and free fatty acid (FFA) species to be significantly increased. Furthermore, LESA-MS was able to successfully differentiate between simple steatosis and more severe NASH, based on a set of short-chain TAGs and FFAs. We compared the data obtained by LESA-MS to that from liquid chromatography (LC)-MS and matrix-assisted laser desorption ionization MS. Advantages of LESA-MS include rapid analysis, minimal sample preparation, and high lipid coverage. Furthermore, since tissue slices are routinely used for diagnostics in clinical settings, LESA-MS is ideally placed to complement traditional histology. Overall LESA-MS is found to be a robust, fast, and discriminating approach for determining NAFLD presence and severity in clinical samples.

Published

2017