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Characterization of Protein Sumoylation in Response to Alkylation Stress in HEK 293 CellsManza, Linda Lee January 2007 (has links)
Stress conditions such as heat shock, UV, alkylating agents, and H2O2 have been shown to result in the modification of a variety of protein targets via the production of reactive electrophiles. These modifications can directly impact protein function or can alter posttranslational modifications, thus leading to a disruption of cellular regulatory processes. Recent studies have shown that stress-induced protein modifications can modulate posttranslational modification by the small ubiquitin related modifier (SUMO) family of proteins. Unlike ubiquitination, which primarily targets proteins for proteasomal degradation, sumoylation exerts a variety of effects including protein stabilization, subcellular localization, and the alteration of protein-protein interactions and transcriptional activity. To investigate the effects of alkylation and oxidative stress on sumoylation, HEK293 cells were treated with iodoacetamide, hydroquinone, benzoquinone, Texas Red C5 bromoacetamide, hydrogen peroxide, and 4-hydroxynonenal (HNE), a highly reactive product of lipid peroxidation associated with oxidative stress. Western blot analysis revealed that the agents tested resulted in concentration-dependent changes in the patterns of SUMO-1 and SUMO-2/3 protein conjugation. Localization studies using western blot analysis and confocal immunofluorescence microscopy demonstrated that SUMO-1 protein conjugates were located primarily in the nucleus, whereas SUMO-2/3 protein conjugates were more equally distributed between the nucleus and the cytoplasm. SUMO-associated proteins were harvested from vehicle- and HNE-treated non-transfected HEK293 cells using agarose conjugated anti-SUMO-1 antibodies or from HA-SUMO-1- and HA-SUMO-3-expressing HEK293 cells using immunoaffinity chromatography. Multidimensional liquid chromatography-tandem mass spectrometry analyses resulted in the identification of 54 HA-SUMO-1-associated proteins and 37 HA-SUMO-3-associated proteins in vehicle-treated cells and 21 HA-SUMO-1- and HA-SUMO-3-associated proteins in HNE treated cells. Additionally, 27 SUMO-1-associated proteins were identified in the HNE-treated non-transfected cells. The functional classes of proteins targeted included RNA binding and processing proteins, metabolic enzymes, cytoskeletal regulators, and chaperone proteins. HNE treatment resulted in a near complete redistribution of both SUMO-1 and SUMO-3 to different targets. There was a 15% overlap in SUMO-1 and SUMO-3 associated proteins in vehicle-treated cells and a 10% overlap in HNE-treated cells indicating that SUMO proteins target distinct protein groups. These results indicate that protein modifying reactive electrophiles can regulate protein functions through the indirect alteration of endogenous posttranslational modifications.
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Resíduos de agrotóxicos em água potável usando SPE e determinação rápida por LC-MS/MS e GC-MS/MS / Pesticide residues in drinking water using SPE and rapid determination by GC-MS/MS and LC-MS/MSDonato, Filipe Fagan 31 August 2012 (has links)
Conselho Nacional de Desenvolvimento Científico e Tecnológico / The use of pesticides always has been associated with the effective control of pests
or invasive weeds to ensure an increase in the food production. However, the indiscriminate
use of these substances has caused the degradation of water resources. In Brazil, the
Ministry of Health through Ordinance 2914 defines several parameters of potability, among
them, the maximum limits allowed for same pesticides. In this work it was developed and
validated a method for the determination of residues of 70 pesticides in drinking water using
(SPE) for sample preparation and determination by Gas and Liquid Chromatography coupled
to tandem mass spectrometry, triple quadrupole analyzer (GC-(TQ)MS/MS and LC-
(TQ)MS/MS). It was evaluated different sample volume, sorbents and solvent of elution. The
best results were obtained using 100 mL sample acidified at pH 2.5, Oasis® SPE cartridge
HLB 60 mg/3 mL and dichloromethane/methanol as eluent. Analytical curves were linear
between 10 and 250 Sg L-1, with r2 values greater than 0.99 for all compounds. The values of
method LOQ were 0.02 Sg L-1 for aldrin, dieldrin and chlordane and 0.5 Sg L-1 for the other
compounds. To evaluate accuracy the blank samples ware fortified at 0.5, 1.5 and 4.0 Sg L-
1 and an extra level at 0.02 Sg L-1 for aldrin, dieldrin and chlordane. The method showed
good precision, with RSD values below to 20% and good accuracy, with recoveries between
70 and 120%. Only the compounds methamidophos, aldicarb, benfuracarb, terbufos,
benomyl and thiophanate methyl were not recovered adequately. The matrix effect was
evaluated, showing upper 10% for the most compounds. In order to compensate this effect,
analytical curves were obtained with standarts prepared in blank extracts of the matrix. The
validated method was applied to 12 samples of drinking water of different characteristics
(river, shed, well and treated water), and just one of the river samples presented residues of
lambda-cyhalothrin. The results indicate that the proposed method is suitable for analysis of
pesticides residues in drinking water, since all the validation parameters met the suggested
limits and parameters for validation of chromatographic methods. / O uso de agrotóxicos sempre esteve associado à efetividade no controle de pragas
ou plantas invasoras para aumentar a produção de alimentos. No entanto, o uso
indiscriminado dessas substâncias vem causando a degradação dos recursos hídricos. No
Brasil, o Ministério da Saúde através da Portaria 2914 define diversos parâmetros de
potabilidade, entre eles, os limites máximos permitidos para alguns agrotóxicos. No presente
trabalho foi desenvolvido e validado um método para a determinação de resíduos de 70
agrotóxicos em água potável, utilizando Extração em Fase Sólida (SPE) para o preparo de
amostra e determinação por Cromatografia Gasosa e Líquida, acopladas à Espectrometria
de Massas sequencial, com analisador triplo quadrupolo (GC-(TQ)MS/MS e LC-
(TQ)MS/MS). Foram avaliados diferentes volumes de amostra, sorventes e solventes de
eluição. Os melhores resultados foram obtidos com 100 mL de amostra acidificada em pH
2,5, cartucho SPE Oasis® HLB 60 mg/3 mL e diclorometano/metanol como eluente. As
curvas analíticas apresentaram linearidade entre 10 e 250 Sg L-1, com valores de r2 maiores
que 0,99 para todos os compostos. Os valores de LOQ do método foram 0,02 Sg L-1 para
aldrin, dieldrin e clordano e de 0,5 Sg L-1 para os demais compostos. Para avaliação da
exatidão as amostras branco foram fortificadas em 0,5, 1,5 e 4,0 Sg L-1 e um nível extra em
0,02 Sg L-1 para os compostos aldrin, dieldrin e clordano. O método apresentou boa
precisão, com valores de RSD inferiores a 20% e boa exatidão, com recuperações entre 70
e 120%. Apenas os compostos metamidofós, aldicarbe, benfuracarbe, terbufós, benomil e
tiofanato metílico não foram recuperados de forma adequada. O efeito matriz foi avaliado,
mostrando-se superior a 10% para a maioria dos compostos. A fim de compensar este
efeito, utilizou-se curvas analíticas preparadas no extrato branco da matriz. O método
validado foi aplicado em 12 amostras de água potável de diferentes características (rio,
vertente, poço e água tratada), sendo que apenas uma das amostras de água de rio
apresentou resíduos de lambda-cialotrina. Os resultados indicam que o método proposto é
adequado à análise de resíduos de agrotóxicos em água potável, visto que todos os
parâmetros de validação atenderam os limites e parâmetros sugeridos para validação de
métodos cromatográficos.
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Lipidome LC/MS Analysis in the Insect Adaptation and Development Studies / Lipidome LC/MS Analysis in the Insect Adaptation and Development StudiesTOMČALA, Aleš January 2009 (has links)
Insects represent very useful experimental model in various branches of biological research. The investigation is driven by economic importance of many insect species, and also by biological features of insects as model organisms such as short period of reproduction, easy breeding and manipulation and, in particular, the minimal regulatory requirements which are associated to the management of vertebrates. Here we report robust and efficient LC/MS/MS methodology for the determination of the physiologically important lipid molecular species in insects. The target metabolites represent polar glycerophos-phopholipids (GPL) and nonpolar lipids diacylglycerols (DG) and triacylglycerols (TG). Combination of the LC/MS data with the subsequent GC fatty acid analysis enables complete structural elucidation of particular lipid species including their fatty acid compositions. The developed methodology was applied to studies of the chill tolerance of the firebug Pyrhocorris appterus. Fields and laboratory experiments were conducted to separate the triggering effects of low temperature, desiccation and diapause progression on the physiological characteristics related to chill tolerance with emphasis on the restructuring of GPL composition. The same effect on the GPL composition was observed during acclimatization in the field and cold acclimation in laboratory. By contrast, the GPL changes related to desiccation and diapause progression were relatively small (Tomčala et al, 2006). In adults of Drosophila melanogaster it has been found that acclimation at 15, 20 and 25°C during preimaginal development affects thermal tolerance and composition of membrane GPLs. Low temperature acclimation was associated with increase in proportion of ethanolamine at the expense of choline in GPLS. Relatively small, but statistically significant changes in lipid molecular compositon were observed with decreasing acclimation temperature (Overgard et al, 2008). Hormonal treatment studies on insect model Locusta migratoria showed a heterogeneous distribution of individual DGs in haemolymph after the hormone application and revealed that mobilization of the DGs is molecular species-specific with the highest proportion of DG 16:0/18:1 and forming in summary about 20% of the total mobilized DG content. Additional analysis of fat body triacylglycerols revealed that the AKH mobilizes the DGs specifically with the preference of those possessing the unsaturated C18 fatty acids (FAs). The fat body FAs with more than 18 carbons did not participate on the mobilization (Tomcala et al, 2009). The LC/MS methodology was further applied to lipid composition studies of several samples with very diverse biological origin (fish, human blood etc.) and was proved to be universally applicable to the wide scope of biological samples.
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Quantification of Isradipine in Human Plasma Using LC-MS/MS for Pharmacokinetic and Bioequivalence StudyPark, Jin H., Park, Yoo Sin, Rhim, Si Y., Jhee, Ok H., Kim, Shin H., Yang, Seok C., Lee, Min H., Shaw, Leslie M., Kang, Ju S. 01 January 2009 (has links)
A highly sensitive and rapid method for the analysis of isradipine in human plasma using liquid chromatography coupled to tandem mass spectrometry (LC-MS/MS) was developed. The procedure involves a simple liquid-liquid extraction of isradipine and amlodipine (IS, internal standard) with methyl-t-butyl ether after alkaline treatment and separation by RP-HPLC. Detection was performed by positive ion electrospray ionization (ESI) in multiple reaction monitoring (MRM) mode, monitoring the transitions m/z 372.1 → m/z 312.2 and m/z 408.8 → m/z 237.9, for quantification of isradipine and IS, respectively. The standard calibration curves showed good linearity within the range of 10 to 5000 pg/mL (r2 ≥ 0.9998). The lower limit of quantitation (LLOQ) was 10 pg/mL. The retention times of isradipine (0.81 min) and IS (0.65 min) suggested the potential for high throughput of the proposed method. In addition, no significant metabolic compounds were found to interfere with the analysis. This method offered good precision and accuracy and was successfully applied for the pharmacokinetic and bioequivalence studies of 5 mg of sustained-release isradipine in 24 healthy Korean volunteers.
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Cílená analýza a metabolismus mastných kyselin u myší a lidí / Targeted analysis and metabolism of fatty acids in mice and humansOseeva, Marina January 2021 (has links)
Widespread sedentary lifestyle and unhealthy eating habits in the last few decades have resulted in a dramatic increase of the number of people affected by obesity, type 2 diabetes, and cardiovascular diseases. The study of these pathological conditions revealed that impaired metabolism often causes these disorders. Lipid metabolism research has contributed significantly to determining mechanisms underlying metabolic disorders. Omega-3 fatty acids are an interesting target for lipidomics studies because they were shown to lower risk of cardiovascular diseases and are hypothesized to regulate lipid metabolism. In this work, I optimized lipid extraction and chemical modification methods for analysis of fatty acids profile of tissue samples and biofluids using comprehensive two-dimensional gas chromatography coupled to mass spectrometry (GCxGC-MS). At first, I evaluated the relative amount of omega-3 fatty acids in red blood cells (Omega-3 index) of people living in Czech Republic in either the capital city (n=476) or the rural region (n=388). For this large-scale project, I extracted phospholipids from red blood cell (RBC) membranes, transesterified them into fatty acid methyl esters (FAMEs), and measured their profile by GCxGC-MS. The mean Omega-3 index was 3.56 mol % and I detected no significant...
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Simultaneous Tissue Extraction and Quantification of Reproductive Neuropeptides and Sex Steroids in Zebrafish and MouseLu, Chunyu 19 August 2022 (has links)
The detection and quantification of hormones are important to assess the reproductive and stress status of experimental models and for the diagnosis of diseases in human and veterinary clinics. The peptide secretoneurin (SN) has been proposed as a new sex hormone, but effective quantification methods are challenging. Traditional methods require the use of antibodies with either radioactive or non-radioactive tracers. There are difficulties with these methods in terms of sensitivity, specificity, and inter-laboratory repeatability. Liquid chromatography-tandem mass spectrometry (LC-MS/MS) can circumvent many of these challenges. Another source of variation is the extraction of lipophilic steroidal compounds, which is incompatible with the extraction of hydrophilic peptide hormones. I have developed efficient extraction and sensitive detection methods of SN with numerous other peptide and steroid hormones in the same tissue sample in mice and zebrafish. The extraction efficiency for both peptide and steroid analytes is over 85%. The standard deviation for extraction and LC-MS/MS analysis for each compound varies between 5-10%. The steroid hormones can be quantified in the low to medium fmol/µL range. We quantified peptide hormones in the high fmol/µL to low pmol/µL range. Mouse SN levels were measured and compared against the levels of GnRH 1, oxytocin, vasopressin, E2, and P4 in multiple tissues at 3 important periods through the estrous cycle. In addition, SN levels were found to be moderately related to GnRH 1 levels in the hypothalamus in the estrous cycle. This is important because it is GnRH 1 that stimulates the luteinizing hormone surge in the pituitary that regulates ovulation in all vertebrate species. I also determined that SNa and SNb were both within the 2-8 pmol/µL range in the brain or pituitary harvested from a single female zebrafish. This makes it feasible for the first time to study the correlation between the SNs and other peptides and steroid hormones by quantifying them simultaneously in very small tissue samples. Untargeted peptidomics determined that the SN peptides in zebrafish can be further processed into smaller discrete fragments. This implies not only active synthesis and selective peptide processing but suggests that the are unknown functions of the SN peptide fragments that await discovery. This cost-effective package was used for the detailed assessment of hypothalamic-pituitary-gonadal function in mice and zebrafish and may be adaptable to many other hormones across species.
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Implementing an LC-QQQ method for the quantification of vitamin D analogues from serum accounting for epimers and isobars / Jacobus Cornelius van der WesthuizenVan der Westhuizen, Jacobus Cornelius January 2014 (has links)
In the early 19th century a ground-breaking discovery was made that linked a dietary
deficiency of a fat-soluble vitamin with the childhood disease known as rickets. The vitamin
was named vitamin D and extensive research regarding the physiological importance of this
vitamin followed ever since. It is currently known that vitamin D plays an important role in
maintaining the calcium and phosphate homeostasis in the human body. Less clear
evidence states the medical importance of vitamin D in the prevention and cancer,
autoimmune disease and diabetes. Current literature shows that vitamin D has five distinct
forms, vitamin D1 to D5, of which vitamin D2 and D3 are the most studied forms. The term
“vitamin D” is often wrongfully used to include the vitamin D mother molecule, the vitamin D
status indicator (25(OH)D), the biologically active form (1,25(OH)2D) and biologically inactive
form (24,25(OH)2D). The interest for measurement of these vitamin D analogues is a
continuously growing field both on individual and epidemiological level. For decades
laboratories have struggled to produce a robust method capable of quantifying these
different vitamin D analogues and uncovered a new form of complexity regarding the
analysis of these analogues. The identification of the C3-epimeric forms of vitamin D
metabolites has forced laboratories to rethink their analytical methods and several concerns
were raised regarding the overestimation of the true vitamin D status by current analytical
methods. The quantification of the biologically active and inactive forms of vitamin D is
reported to be difficult and to date very few LC-MS/MS methods reported in the literature are
able to quantify various vitamin D analogues. However, to our knowledge none of these
methods are able to include the precursor vitamin D, the 25-hydroxylated metabolites, the
biologically active and inactive metabolites, C3-epimers and isobaric compounds in a single
run.
Therefore the aim of this study was to develop, optimise and validate a LC-MS/MS method
for the quantification of twelve vitamin D analogues in a single run. This was done by
optimising the underlying LC-MS/MS parameters to ensure optimal analytical sensitivity in
positive ESI mode and sufficient chromatographic separation between analytes with similar
chemical properties. Furthermore, the optimised method was validated to ensure the
accuracy and precision of the method before implementation into a clinical environment. The
vitamin D analogues included in this study were vitamin D2, vitamin D3, 25(OH)D2,
25(OH)D3, 1,25(OH)2D2, 1,25(OH)2D3, 24,25(OH)2D2, 24,25(OH)2D3, 3-epi-25(OH)D2, 3-epi-
25(OH)D3, 7(OH)4C3 and 1α(OH)D3.
A double liquid-liquid extraction with hexane and ethyl acetate were found to be the most
efficient at extracting the vitamin D analogues from a serum matrix after matrix modification with sodium hydroxide. Recoveries of > 95 % (CV <10 %) were achieved for all the analytes.
It was noted that a precursor adduct other than the molecular mass ion for a specific vitamin
D analogue can produce a more abundant MS1 signal and that the ESI source parameters
vary between analytes with different chemical properties and should therefore be optimised
individually for each analyte. Various columns were assessed and sufficient
chromatographic separation between the relevant analytes was achieved with an Agilent
Technologies Pentafluorophenyl column. Baseline separation was achieved between
25(OH)D3 and 3-epi-25(OH)D3 as well as 25(OH)D2 and 3-epi-25(OH)D2, which is a
requirement for this method to be viable. The method was subjected to a series of validation
steps to ensure the accuracy and precision of the method. These included the assessment
of the analytical range, LOD, LOQ, inaccuracy, imprecision, stability, interference and
recovery. It was found that the optimised method had good linearity (r > 0.995), acceptable
repeatability (CV < 10 %) and within-lab precision (CV < 15%) and excellent method
accuracy (systematic error < 6.60 %). Furthermore, all the analytes proved to be stable for
48 hours after sample preparation with no interferences found for co-eluting analytes.
Finally, based on the sigma metric scale specifications, it was calculated that this method
proved to be “world class” and very little QC is needed to ensure the quality of the data
derived from this method.
Based on the findings in this study, it was concluded that a novel LC-MS/MS method for the
quantification of twelve vitamin D analogues in a single run was successfully developed. All
the LC-MS/MS parameters were optimised to ensure optimal analytical sensitivity for each
analyte and the method was validated based on a series of method validation steps required
for implementation into a clinical laboratory. This validation proved this method to be ready
for implementation into a clinical environment. / MSc (Biochemistry), North-West University, Potchefstroom Campus, 2015
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Implementing an LC-QQQ method for the quantification of vitamin D analogues from serum accounting for epimers and isobars / Jacobus Cornelius van der WesthuizenVan der Westhuizen, Jacobus Cornelius January 2014 (has links)
In the early 19th century a ground-breaking discovery was made that linked a dietary
deficiency of a fat-soluble vitamin with the childhood disease known as rickets. The vitamin
was named vitamin D and extensive research regarding the physiological importance of this
vitamin followed ever since. It is currently known that vitamin D plays an important role in
maintaining the calcium and phosphate homeostasis in the human body. Less clear
evidence states the medical importance of vitamin D in the prevention and cancer,
autoimmune disease and diabetes. Current literature shows that vitamin D has five distinct
forms, vitamin D1 to D5, of which vitamin D2 and D3 are the most studied forms. The term
“vitamin D” is often wrongfully used to include the vitamin D mother molecule, the vitamin D
status indicator (25(OH)D), the biologically active form (1,25(OH)2D) and biologically inactive
form (24,25(OH)2D). The interest for measurement of these vitamin D analogues is a
continuously growing field both on individual and epidemiological level. For decades
laboratories have struggled to produce a robust method capable of quantifying these
different vitamin D analogues and uncovered a new form of complexity regarding the
analysis of these analogues. The identification of the C3-epimeric forms of vitamin D
metabolites has forced laboratories to rethink their analytical methods and several concerns
were raised regarding the overestimation of the true vitamin D status by current analytical
methods. The quantification of the biologically active and inactive forms of vitamin D is
reported to be difficult and to date very few LC-MS/MS methods reported in the literature are
able to quantify various vitamin D analogues. However, to our knowledge none of these
methods are able to include the precursor vitamin D, the 25-hydroxylated metabolites, the
biologically active and inactive metabolites, C3-epimers and isobaric compounds in a single
run.
Therefore the aim of this study was to develop, optimise and validate a LC-MS/MS method
for the quantification of twelve vitamin D analogues in a single run. This was done by
optimising the underlying LC-MS/MS parameters to ensure optimal analytical sensitivity in
positive ESI mode and sufficient chromatographic separation between analytes with similar
chemical properties. Furthermore, the optimised method was validated to ensure the
accuracy and precision of the method before implementation into a clinical environment. The
vitamin D analogues included in this study were vitamin D2, vitamin D3, 25(OH)D2,
25(OH)D3, 1,25(OH)2D2, 1,25(OH)2D3, 24,25(OH)2D2, 24,25(OH)2D3, 3-epi-25(OH)D2, 3-epi-
25(OH)D3, 7(OH)4C3 and 1α(OH)D3.
A double liquid-liquid extraction with hexane and ethyl acetate were found to be the most
efficient at extracting the vitamin D analogues from a serum matrix after matrix modification with sodium hydroxide. Recoveries of > 95 % (CV <10 %) were achieved for all the analytes.
It was noted that a precursor adduct other than the molecular mass ion for a specific vitamin
D analogue can produce a more abundant MS1 signal and that the ESI source parameters
vary between analytes with different chemical properties and should therefore be optimised
individually for each analyte. Various columns were assessed and sufficient
chromatographic separation between the relevant analytes was achieved with an Agilent
Technologies Pentafluorophenyl column. Baseline separation was achieved between
25(OH)D3 and 3-epi-25(OH)D3 as well as 25(OH)D2 and 3-epi-25(OH)D2, which is a
requirement for this method to be viable. The method was subjected to a series of validation
steps to ensure the accuracy and precision of the method. These included the assessment
of the analytical range, LOD, LOQ, inaccuracy, imprecision, stability, interference and
recovery. It was found that the optimised method had good linearity (r > 0.995), acceptable
repeatability (CV < 10 %) and within-lab precision (CV < 15%) and excellent method
accuracy (systematic error < 6.60 %). Furthermore, all the analytes proved to be stable for
48 hours after sample preparation with no interferences found for co-eluting analytes.
Finally, based on the sigma metric scale specifications, it was calculated that this method
proved to be “world class” and very little QC is needed to ensure the quality of the data
derived from this method.
Based on the findings in this study, it was concluded that a novel LC-MS/MS method for the
quantification of twelve vitamin D analogues in a single run was successfully developed. All
the LC-MS/MS parameters were optimised to ensure optimal analytical sensitivity for each
analyte and the method was validated based on a series of method validation steps required
for implementation into a clinical laboratory. This validation proved this method to be ready
for implementation into a clinical environment. / MSc (Biochemistry), North-West University, Potchefstroom Campus, 2015
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Förhållandet mellan förändrat självkoncept och personlig identitet vid livsförändringar : Om MS sjukaLisa, Lewin January 2008 (has links)
<p>Under en individs liv erfars i regel många livsomvälvande händelser som fungerar förändrande och utvecklande. I vissa fall leder en företeelse till att en individs identitet genomgår en förändring. Denna studies fokus riktas mot förhållandet mellan ett reviderat självkoncept och den personliga identiteten. En kvalitativ metod genomfördes där åtta individer med sjukdomen MS intervjuades. Studien visade att intervjupersonernas upplevelse av den egna kroppen, sig själva och de värderingar de attribuerade till sig själva, det vill säga självkonceptet, förändrades till följd av de hinder och begränsningar sjukdomen bidragit till. Detta fick till följd att den personliga identiteten omskapades i fråga om karaktärsdrag och målsättningar. Studien bidrar med fördjupade kunskaper om förändringar i självkonceptet och den personliga identiteten vid sjukdom.</p> / <p>During an individual’s life many events develop and change the person and some may even change the individuals’ identity. Focusing on the relationship between an altered self-concept and the personal identity, a qualitative attempt was made. Eight interviews were made with individuals who suffered from MS. The result showed that the way the participants experienced themselves, their bodies and the way they attributed themselves changed dependent on the obstacles and limitations the disease contributed to. This was followed by changes in the personal identity in terms of characteristics and goals. The study contributes with advanced knowledge about alterations of the self-concept and the personal identity concerning illness.</p>
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Sample introduction into inductively coupled plasma mass spectrometryLofthouse, Simon D. January 1999 (has links)
No description available.
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