Tesis sobre el tema "Sandwich assays"
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Yousef, Jamil. "Development of Sandwich Assays for Potential Protein Biomarkers in Neurodegenerative Diseases". Thesis, KTH, Skolan för kemi, bioteknologi och hälsa (CBH), 2020. http://urn.kb.se/resolve?urn=urn:nbn:se:kth:diva-278727.
Texto completoPrevalensen av neurodegenerativa sjukdomar såsom Alzheimers sjukdom (AD), Parkinsonssjukdom (PD), frontallobsdemens (FTD) och amyotrofisk lateralskleros (ALS) ökar i takt med denåldrande populationen. Pålitliga biomarkörer som kan hjälpa till vid diagnostiseringen av dessasjukdomar behövs för att starta rätt behandling så tidigt som möjligt. Ryggmärgsvätska, enkroppsvätska tillhörande det centrala nervsystemet, kan ge en inblick i det centrala nervsystemetstillstånd. Förändrade proteinnivåer i denna kroppsvätska skulle därför kunna fungera sombiomarkörer. Målet i detta projekt var att validera tidigare föreslagna proteinbiomarkörer iryggmärgsvätska. Utifrån en lista av 80 tidigare analyserade proteiner i ryggmärgsvätska hospatienter, inkluderades åtta proteiner i detta valideringsförsök. En antikroppsbaserad så kalladsandwich assay användes i en suspension bead array för att testa 21 stycken antikroppar i ett initialtscreeningsförsök. Antikroppspar som kunde mäta proteinnivåer på ett spädningsberoende vis i detinitiala screeningsförsöket optimerades vidare innan den utvecklade sandwich assayn användes föratt analysera proteinnivåer i individuella prover. Sandwich assays gentemot Amphiphysin(AMPH), Chitotriosidase-1 (CHIT1) och Beta-synuclein (SNCB) kunde bli framtagna ochkorrelerade gentemot tidigare genererat data från en single binder assay på ett framgångsrikt sätt.Projektet kunde därmed validera tidigare fynd som indikerat förhöjda nivåer av AMPH och SNCBi AD patienter, samt förhöjda nivåer av CHIT1 i ALS patienter.
Marten, Katharina [Verfasser] y Anil [Akademischer Betreuer] Batra. "Entwicklung eines Sandwich Enzyme-linked Immunosorbent Assays zum Nachweis von humanem α-Synuclein / Katharina Marten ; Betreuer: Anil Batra". Tübingen : Universitätsbibliothek Tübingen, 2017. http://d-nb.info/119954728X/34.
Texto completoJana, Subha. "Biodetection using fluorescence energy transfer from Quantum dot excited whispering gallery modes to fluorescent acceptors". Electronic Thesis or Diss., Université Paris sciences et lettres, 2021. http://www.theses.fr/2021UPSLS081.
Texto completoQuantification of specific biomarkers is an important diagnostic tool. Standard immunoassays such as ELISA require extensive washing steps and signal amplification, in particular when the biomarker of interest is only present at very low concentrations. On the other hand, non-radiative Förster resonance energy transfer (FRET) has been used to design one-step homogenous bioassays which do not require any washing steps, where the biomarker enables the formation of a sandwich complex involving donor-labeled and acceptor-labeled antibodies. FRET from the donor to the acceptor then provides an optical signature of the complex formation, hence of the biomarker of interest. However, FRET which is highly sensitive to the donor-acceptor distance, only occurs in a significant rate when the distance between the donor and acceptor is less than 10 nanometers; thus the large size of many biological complexes limits the efficiency of energy transfer, preventing sensitive detection. Here I propose a novel energy transfer modality that uses solution-phase optical microcavities to enhance energy transfer. Following that, I describe a bio-sensing scheme designed to detect a cancer biomarker DNA in solution.To this aim, I have designed microcavity structures in which fluorescent colloidal quantum dots are located inside dielectric polymer microspheres to enable strong coupling of their fluorescence emission with the cavity resonance modes or whispering gallery modes (WGMs) of the microspheres. A detailed study was carried out to comprehend the structural and optical properties of these optical microcavities. I also characterized the energy transfer between these modes and acceptor dye-loaded nanoparticles present in the evanescent field, within a few tens of nanometers above the microsphere surface. An analytical model was constructed to provide insights into the WGM mediated energy transfer (WGET) mechanisms. Moreover, a comparison between WGET and FRET revealed the superiority of WGET in the context of building sensors with improved sensitivity and longer range of detection. In the last part of the thesis, a strategy is discussed in detail to provide biological functionalities to these optical microcavities which would enable them to interact with target analytes such as DNA, RNA, and proteins with high specificity, and moreover to reduce non-specific interactions. This strategy then was adapted to attach DNA capture probes onto the WGM enabled microcavities. Using the DNA attached microspheres as optical donor in combination with probe-DNA functionalized dye nanoparticles as optical acceptors, a biosensing assay has been successfully demonstrated to detect a cancer biomarker DNA called survivin in the solution phase. This assay did not only show good sensitivity towards the target, but also it has proven to be highly specific. The detection scheme has been demonstrated in a sophisticated confocal microscope at the single microsphere level, then successfully translated to a much simpler spectrofluorometer that measures fluorescence from the whole sample solution; the signature of the sandwich complex formation was also effectively detected.In conclusion, I demonstrated that microcavity-assisted energy transfer has several advantages over regular FRET assays. A real bio-sensing assay based on the WGET principle has also been successfully designed to detect cancer biomarkers with high sensitivity and specificity. This study thus opens up many possibilities to design high-performing and more accurate assays to detect varieties of biological entities
Bregulla, Julie. "Investigation into the fire and racking behaviour of structural sandwich panel walls : a methodology to assess load bearing sandwich panels in fire". Thesis, University of Surrey, 2003. http://epubs.surrey.ac.uk/807/.
Texto completoLima, Jefferson Queiroz. "Contribution to knowledge chemical plant of gender Tephrosia: Chemical investigation and biological assays of Tephrosia egregia Sandwith (Fabaceae)". Universidade Federal do CearÃ, 2010. http://www.teses.ufc.br/tde_busca/arquivo.php?codArquivo=4658.
Texto completoThe present work describes the chemical study of leaves, stems and roots of the Tephrosia egregia Sandwith (Fabaceae) species, through the analysis of the volatile and nonvolatile constituent of the specie. The determination of the volatile chemical composition of leaves and stems of T. egregia showed the predominance of sesquiterpenes, with some monoterpenes and trisnor-sesquiterpenes. The comparison between identified constituents in the leaves (16; 88.75%) and stems (13; 85.22%) showed a similarity between the samples, although the trisnor-sesquiterpenes geijeren and pregeijeren were the major constituents in both the essential oils. From the chromatographic investigation of the essential oil of leaves, the trisnor-sesquiterpene dictamnol was isolated for the first time in the Tephrosia genus. The chromatographic investigation of the roots of T. egregia yields pongachalcone and praecansone B, of pongaflavone, of 6a,12a-dehydrorotenone and 12a-hydroxyrotenone, the mixture of sitosterol and stigmasterol, and their glucosylated forms, and the maackiain. From its leaves were isolated p-coumaric acid and ferulic acid. This two compounds had been isolated for the first time in the genus. The assays with extracts and isolated substances of T. egregia showed that the studied specie has very important larvicidal activity against Aedes aegypti and allelopathic activity, with best result for the ethanolic extract of the roots. In other hand, the bioassays of antimicrobial activity against of S. aureaus, E. coli, P. aeruginosa, S. choleraesuis and C. albicans, and the nematicidal activity on Meloidogyne incognta not shown significant results.
O presente trabalho descreve o estudo quÃmico das folhas, talos e raÃzes de Tephrosia egregia Sandwith (Fabaceae), atravÃs da anÃlise dos constituintes volÃteis e nÃo volÃteis da espÃcie. A determinaÃÃo da composiÃÃo quÃmica volÃtil das folhas e talos de T. egregia mostrou a predominÃncia de sesquiterpenos, com relatos de monoterpenos e trisnorsesquiterpenos. A comparaÃÃo entre os constituintes identificados nas folhas (16; 88,75%) e talos (13; 85,22%) revelou semelhanÃa entre os mesmos, onde os trisnor-sesquiterpenos geijereno e o pregeijereno foram os constituintes majoritÃrios em ambos os Ãleos essenciais. A partir do fracionamento cromatogrÃfico do Ãleo essencial das folhas foi isolado o trisnorsesquiterpeno dictamnol, relatado pela primeira vez no gÃnero Tephrosia. O estudo dos constituintes nÃo volÃteis foi iniciado a partir da obtenÃÃo dos extratos etanÃlicos das folhas, talos e raÃzes da espÃcie estudada. O fracionamento cromatogrÃfico das raÃzes levou ao isolamento das chalconas pongachalcona e praecansona B, da flavona pongaflavona, dos rotenoides 6a,12a-desidrorotenona e 12a-hidroxirotenona, da mistura dos esterÃides sitosterol e estigmasterol e de suas misturas nas formas glicosiladas e do pterocarpano maackiaina. A partir do extrato acetato de etila do decocto das folhas de T. egregia foram isolados os fenilpropanÃides Ãcido p-cumÃrico e Ãcido ferÃlico, descritos pela primeira vez no gÃnero estudado. Os ensaios de atividades biolÃgicas realizados para os extratos e substÃncias isoladas de T. egregia mostraram que a espÃcie estudada apresenta atividades larvicida sobre Aedes aegypti e alelopÃtica significativas, com destaque para o extrato etanolico das raÃzes (TERES). NÃo foram encontrados resultados significativos para os bioensaios de atividade antimicrobiana sobre cepas de S. aureaus, E. coli, P. aeruginosa, S. choleraesuis e C. albicans, assim como para atividade nematicida sobre Meloidogyne incognita.
Marassa, Ana Maria. "Identificação de fonte sanguínea em dípteros da Família Culicidae, em áreas de epizootia da febre amarela silvestre". Universidade de São Paulo, 2009. http://www.teses.usp.br/teses/disponiveis/6/6132/tde-20072009-153444/.
Texto completoThe knowledge of mosquitoes Culicidae host feeding patterns permits to clarify some aspects related to zoonosis transmission and to estimate the degree of human-vector contact which is relevant in epidemiological studies. Aiming to explore the feeding behavior of these mosquitoes, specimens were collected in the municipalities of Santo Antônio das Missões and Garruchos, Rio Grande do Sul, an epizootic area of sylvatic yellow fever. Engorged females were collected by aspiration from forested areas from September 2005-April 2007 and their blood meals were identified using the avidin-biotin system of immunoenzymatic ELISA capture. Six blood meal sources were tested: bird, cattle, horse, human, monkey and rat. The result achieved with the species-specific IgG1 mAb was unprecedented for mosquito blood meal identification and reinforced the sensibility and specificity of the immunoenzymatic ELISA capture. Of the 190 samples from Santo Antônio das Missões, 60.9% reacted to cattle, 23.6% to human, 9.9% to bird, 1.9% to monkey and 3.7% to mixed blood meals. In Garruchos, of the 158 females collected in Cachoeirinha, 16.0% reacted to bird, 29.6% to cattle, 36.8% to human, 4.0% to horse, 0.8% to monkey and 12.8% to mixed blood, while of the 149 engorged females from São José, blood from cattle accounted for 51.5%, of blood identified, bird and human 11.5%, monkey 6.2%, horse 0.8% and mixed blood 18.5%. Blood engorged females of Aedes scapularis, Aedes crinifer, Culex (Culex) spp., Haemagogus leucocelaenus predominated in the two municipalities. The results obtained with Aedes scapularis suggests its eclecticism, according to the combinations of blood which were detected from different sources. Haemagogus leucocelaenus was found to have the highest proportion of samples containing human blood in comparison with other sources, which has implications, on account of being incriminated in the transmission and also for taking into consideration the outbreaks reported that underline the risk of yellow fever.
Liebenberg, Annerie. "The development of an enzyme linked immunosorbent assay for the detection of the South African strain(s) of grapevine fanleaf nepovirus". Thesis, Link to the online version, 2008. http://hdl.handle.net/10019/1909.
Texto completoParasar, Parveen. "Determination of the Expression Patterns of Bovine Non-Classical Major Histocompatibility Complex (MHC) Class I Proteins". DigitalCommons@USU, 2013. http://digitalcommons.usu.edu/etd/1999.
Texto completoLeón, janampa Nancy. "Development of a test associated with magnetic nanoparticles for the diagnosis of tuberculosis". Thesis, Bordeaux, 2019. http://www.theses.fr/2019BORD0272.
Texto completoMycobacterium tuberculosis causes one of the diseases with the highest mortality and morbidity rate in the Americas and around the world. In developing countries, the diagnosis of tuberculosis (TB) is based on smear microscopy and bacteriological cultures. The first method has low sensitivity, and the second take several weeks to reach a confirmatory diagnosis. The lack of a rapid diagnosis compromises the efforts to control TB, favoring its transmission to the susceptible population. Currently, magnetic nanoparticles (MNPs) functionalized with biomolecules have been used in biomedicine, due the magnetic, electrical and optical properties. In this way, applying external magnetic fields, bio-functionalized MNPs is used to detect and concentrate cells and biomolecules from biological samples.In this work we present the synthesis, characterization and bio-functionalization of magnetic nanoparticles, to develop a sandwich ELISA assay associated to MNPs to detect antigens from M. tuberculosis. For this purpose, magnetic nanoparticles were synthesized by co-precipitation method. The MNP surface was amine-silanized (MNP@Si@NH2) and characterized by physical-chemical methods.The MTB antigens evaluated in this study were: Hsp16.3, CFP10, ESAT6, MTC28, MPT64, 38 kDa protein, Ag85B and MoeX. Cloning ad expression of recombinant proteins were made in E. coli BL21 (DE3) pLysS system. Polyclonal antibodies were produced in New Zealand rabbits and BALB/C mice, previously immunized with purified recombinant antigens. Specific antibodies (ab) were immobilized in the amine-silanized MNP surfaces. The MNP@Si@ab were associated in a colorimetric sandwich ELISA assay to capture and detect native MTB antigens from sputum samples.The XRD, Mössbauer spectroscopy, zeta potential, TEM and FTIR demonstrated the successful preparation of the MNPs showing a diffraction crystal diameter of ~12.5 nm (10.48 ± 2.56 nm), superficial net charge of ᶎ: +23.57 ± 2.87 mV, characteristic patterns of magnetite and a spherical structure. Additionally, a magnetization saturation of 37.06 emu.g-1 was observed. For the functionalization of nanoparticle surfaces with antibodies, active ester method (coupling agent EDC/NHS) were used for peptide bond formation. Parameters such as time of incubation, concentration of coupling agents and surface saturation level of amine-silanized MNPs (MNP@Si@NH2), were previously standardized.Finally, antibody functionalized on MNPs were used to capture and detect recombinant and native M. tuberculosis antigens in an ELISA-MNP@Si@ab sandwich test (in a reaction time <4 h). The ESAT6 and CFP10 antigens were better discriminated in sputum pooles from patients with TB (fold value ~ 1.8). The use of MNP@Si@ab improved the detection of MTB antigens in biological samples. Our results are encouraging, but the essay requires additional evaluations such as determining cross-reactions with sputum samples from patients with other infections, performing the test with fresh sputum of TB patients, and determining the sensitivity and specificity of the method
Mycobacterium tuberculosis causa una de las enfermedades con la tasa más alta de mortalidad y morbilidad en las Américas y en todo el mundo. En países en vías de desarrollo, el diagnóstico de tuberculosis (TB) se basa en microscopía de frotis y cultivos bacteriológicos. El primer método tiene baja sensibilidad y el segundo toma varias semanas para llegar a un diagnóstico confirmatorio. La falta de un diagnóstico rápido compromete los esfuerzos para controlar la TB, lo que favorece su transmisión a la población susceptible. Actualmente, las nanopartículas magnéticas (MNP) funcionalizadas con biomoléculas se han utilizado en biomedicina, debido a las propiedades magnéticas, eléctricas y ópticas. De esta manera, aplicando campos magnéticos externos, se utilizan MNP bio-funcionalizadas para detectar y concentrar células y biomoléculas a partir de muestras biológicas. En este trabajo presentamos la síntesis, caracterización y bio-funcionalización de las nanopartículas magnéticas para desarrollar un ensayo ELISA sándwich usando MNPs para detectar antígenos de M. tuberculosis. Para este propósito, las nanopartículas magnéticas fueron sintetizadas por el método de co-precipitación. La superficie de MNP fue amino-silanizada (MNP@Si@NH2) y se caracterizada por métodos físico y químicos. Los antígenos de MTB evaluados en este estudio fueron: Hsp16.3, CFP10, ESAT6, MTC28, MPT64, proteína de 38 kDa, Ag85B y MoeX. La clonación y la expresión de las proteínas recombinantes se realizaron en el sistema de E. coli BL21 (DE3) pLysS. Se produjeron anticuerpos policlonales en conejos de Nueva Zelanda y ratones BALB/C, inmunizados previamente con antígenos recombinantes purificados. Se inmovilizaron anticuerpos específicos (ab) en las superficies de MNP amino-silanizadas (MNP@Si@ab). El MNP@Si@ab fue utilizado en un ensayo ELISA sándwich colorimétrico para capturar y detectar antígenos de MTB nativos en muestras de esputo. La XRD, espectroscopia de Mössbauer, la potencial zeta, TEM y FTIR demostraron la preparación exitosa de los MNP, el cual mostró un diámetro de difracción del cristal de ~ 12.5 nm (10.48 ± 2.56 nm), carga neta superficial de ᶎ: +23.57 ± 2.87 mV, patrones característicos de magnetita y una estructura esférica. Además, una saturación de magnetización de 37.06 emu.g-1 fue observada. Para la funcionalización de superficies de nanopartículas con anticuerpos, se utilizó el método del éster activo para la formación de enlaces peptídicos. Parámetros tales como el tiempo de incubación, la concentración de los agentes de acoplamiento y el nivel de saturación de la superficie de las MNPs aminosilanizadas (MNP@Si@NH2) fueron estandarizadas. Finalmente, se usaron MNP funcionalizados con anticuerpos para capturar y detectar antígenos nativos y recombinantes de M. tuberculosis en una prueba sándwich de ELISA-MNP@Si@ab en un tiempo de reacción <4 h. Los antígenos ESAT6 y CFP10 se discriminaron mejor en las muestras de esputo de los pacientes con TB (fold value ~ 1,8). El uso de MNP@Si@ab mejoró la detección de antígenos de MTB en muestras biológicas con respecto a un sELISA convencional. Nuestros resultados son alentadores, pero el ensayo requiere evaluaciones adicionales, como determinar reacciones cruzadas con muestras de esputo de pacientes con otras infecciones, realizar la prueba con esputo frescos de pacientes con TB y determinar la sensibilidad y especificidad clînica del método
Pearson, Brooke. "Development of a SERS Sandwich Assay Platform for Rapid Detection of Bacteria". 2017. https://scholarworks.umass.edu/masters_theses_2/529.
Texto completoChen, Qing Nong y 陳清農. "Detection of vibrio parahaemolyticus by digoxigenin labeling colony hybridization assay and quantitative targets for PCR by enzyme-linked oligonucleotide sandwich assay". Thesis, 1994. http://ndltd.ncl.edu.tw/handle/69180957076770625012.
Texto completoFill, Catherine E. "Development of a Novel Lateral-Flow Assay to Detect Yeast Nucleic Acid Sequences". 2012. https://scholarworks.umass.edu/theses/810.
Texto completoLiu, Lihua Hsieh Yun-Hwa Peggy. "Monoclonal antibody-based sandwich ELISA for the detection of ovine muscle in cooked meat". 2006. http://etd.lib.fsu.edu/theses/available/etd-07102006-152630.
Texto completoAdvisor: Yun-Hwa Peggy Hsieh, Florida State University, College of Human Sciences, Dept. of Nutrition, Food and Exercise Sciences. Title and description from dissertation home page (viewed Sept. 19, 2006). Document formatted into pages; contains viii, 75 pages. Includes bibliographical references.
LIN, RONG-PEI y 林榮培. "A sandwich enzyme-linked immunosorbent assay for the detection of antibody and antigen of infectious bursal disease". Thesis, 1991. http://ndltd.ncl.edu.tw/handle/83218487972117180254.
Texto completoTang, Yi-Syuan y 唐翊軒. "Development of a Sandwich Enzyme-Linked Immunosorbent Assay (ELISA) for Porcine Circovirus Type 2 (PCV2) Antigen Detection". Thesis, 2016. http://ndltd.ncl.edu.tw/handle/36287866158602127090.
Texto completo國立宜蘭大學
生物技術與動物科學系
104
Porcine circovirus-associated disease (PCVAD) is an important disease that affects the pig industry, and the major pathogen is Porcine Circovirus type 2 (PCV2). In order to cope with the heavy loss caused by PCV2, leading pharmaceutical and biotech companies have launched PCV2 vaccines and diagnostic reagents. Currently on the market, the diagnostic products for PCV2 detection aim to detect anti-PCV2 antibodies in sera. No commercial products that detect the antigen of PCV2 virus particle are available. The object of this dissertation was to develop an enzyme-linked immunosorbent assay (ELISA) to detect antigens of PCV2. Firstly, monoclonal antibodies against PCV2 virus particle were produced. A large amount of virus obtained from cell culture was purified and used to immunize mice as well as produce hybridomas. After several screenings, a hybridoma cell line, 3A10-D1-H2, capable of secreting antibodies against PCV2 virus particle was successfully isolated. The monoclonal antibodies were verified to recognize PCV2 virus particle by ELISA, indirect immunofluorescence assay (IFA), etc. Purified monoclonal antibodies obtained from murine ascites and rabbit polyclonal antibodies were used to develop an ELISA. Results showed that the sandwich ELISA successfully detected PCV2 viruses produced via cell culture and the sensitivity for purified virus reached ng/ml levels. On the other hand, the monoclonal antibodies produced from this study have the ability to neutralize PCV2 virus infection. The sequence of the high viability zone of PCV2 antibody was also revealed by nucleotide sequence analysis with the hybridoma cell line. The information paves the way for subsequent development of therapeutic chimeric antibodies.
Tseng, Yi Ting y 曾宜婷. "Integrated Microfluidic System for Rapid Detection of the Influenza H1N1 Virus Using a Sandwich-based Aptamer Assay". Thesis, 2015. http://ndltd.ncl.edu.tw/handle/94741391269755714061.
Texto completo國立清華大學
動力機械工程學系
103
The rapid spread of influenza-associated H1N1 viruses has caused serious concern in recent years. Therefore, there is an urgent need for the development of automatic, point-of-care devices for rapid diagnosis of the influenza virus. Conventional approaches suffer from several critical issues; notably, they are time-consuming, labor-intensive, and are characterized by low specificity. In this work, we present a new approach for fluorescence-based detection of the influenza A H1N1 virus using a sandwich-based aptamer assay that is automatically performed on an integrated microfluidic system. The entire detection process was shortened to 30 minutes using this chip-based system, and reagent consumption was decreased 5-fold in comparison to traditional methods. The limit of detection was significantly improved to 0.032 HAU due to the high affinity and high specificity of the H1N1-specific aptamers, suggesting that this microfluidic system could be useful in the detection of the H1N1 virus in situ.
"The development of a sandwich ELISA for grass carp growth hormone and generation of 4 cysteine recombinant grass carp growth hormone". 1998. http://library.cuhk.edu.hk/record=b6073072.
Texto completoThesis (Ph.D.)--Chinese University of Hong Kong, 1998.
Includes bibliographical references (p. 158-168).
Electronic reproduction. Hong Kong : Chinese University of Hong Kong, [2012] System requirements: Adobe Acrobat Reader. Available via World Wide Web.
Mode of access: World Wide Web.
Abstracts in English and Chinese.
Rao, Qinchun Hsieh Yun-Hwa Peggy. "Monoclonal antibody-based sandwich enzyme-linked immunosorbent assay for the detection of mammalian meat in meat and feed products". Diss., 2004. http://etd.lib.fsu.edu/theses/available/etd-07192004-091022/.
Texto completoAdvisor: Dr. Yun-Hwa Peggy Hsieh, Florida State University, College of Human Sciences, Dept. of Nutrition, Food and Exercise Sciences. Title and description from dissertation home page (viewed Apr. 18, 2005). Document formatted into pages; contains ix, 70 pages. Includes bibliographical references.
Soldevila-Barreda, Joan J., Maria Azmanova, Anaïs Pitto-Barry, Patricia A. Cooper, Steven D. Shnyder y Nicolas P. E. Barry. "Preclinical Anticancer Activity of an Electron-Deficient Organoruthenium(II) Complex". 2020. http://hdl.handle.net/10454/18025.
Texto completoRuthenium compounds have been shown to be promising alternatives to platinum(II) drugs. However, their clinical success depends on achieving mechanisms of action that overcome Pt-resistance mechanisms. Electron-deficient organoruthenium complexes are an understudied class of compounds that exhibit unusual reactivity in solution and might offer novel anticancer mechanisms of action. Here, we evaluate the in vitro and in vivo anticancer properties of the electron-deficient organoruthenium complex [(p-cymene)Ru(maleonitriledithiolate)]. This compound is found to be highly cytotoxic: 5 to 60 times more potent than cisplatin towards ovarian (A2780 and A2780cisR), colon (HCT116 p53+/+ and HCT116 p53−/−), and non-small cell lung H460 cancer cell lines. It shows no cross-resistance and is equally cytotoxic to both A2780 and A2780cisR cell lines. Furthermore, unlike cisplatin, the remarkable in vitro antiproliferative activity of this compound appears to be p53-independent. In vivo evaluation in the hollow-fibre assay across a panel of cancer cell types and subcutaneous H460 non-small cell lung cancer xenograft model hints at the activity of the complex. Although the impressive in vitro data are not fully corroborated by the in vivo follow-up, this work is the first preclinical study of electron-deficient half-sandwich complexes and highlights their promise as anticancer drug candidates.
UF150295/Royal Society; University of Bradford; Government Department of Business, Energy and Industrial Strategy; SBF003\1170/British Heart Foundation Springboard Award; AMS_/Academy of Medical Sciences/United Kingdom
"Optimization and Ultimate Limitations for Immunoassay and Clinical Diagnostics". Doctoral diss., 2015. http://hdl.handle.net/2286/R.I.34796.
Texto completoDissertation/Thesis
Doctoral Dissertation Chemistry 2015
Wang, Wan-Pin y 王婉萍. "Development of nenotal kid''s passive and active immunity and the assay of sandwich ELISA applied for the measurement of goat''s immunoglobulin G". Thesis, 1999. http://ndltd.ncl.edu.tw/handle/43461871432168163831.
Texto completo國立中興大學
畜產學系
87
捌、英文摘要 Development of nenotal kid’s passive amd active immunity and the assay of sandwich ELISA applied for the measurement of goat’s immunoglobulin G Waun-Pin Wang Abstract Milk immunoglobulin G (IgG) is main source of immunoglobulin and originates from the blood of ruminant dam. During parturition, the levels of mother blood and milk IgG are distinctly elevated. The newborn kids have low levels of IgG and low titer of innate immunity because the blood IgG of dam is not cross the placenta of dam side. In addition, the gut closure appears within 1-2 day after birth. The colostral IgG is acquired for passive immunity in kids. The present study was conducted to test the ability of passive immunity after kids fed colostrum, heat inactivated colostrum, milk of late lactation or cRBC-induced colostrum. Futhermore, the alterations of serum and colostral IgG in prepartum and postpartum of dams were examined. The bleeding and collecting mammary secretes of dams were at prepartum (-7,-3,-1day), parturition (0day), and postpartum (1,3,7day) respectively. Two dams were immunized with cRBC (s.c) once every week before 4 weeks of parturition. Their kids were fed cRBC-induced colostrum after birth. Normal kids were randomly assigned to feed colostrum, heat inactivated colostrum or milk every 6hr after birth and were bled prior to feeding for 5 consecutive days. The kids were administrated with chicken RBC at 3 and 5 weeks old respectively and were bled once at 6 weeks old. After electrophoresis and electroelution, the purified goat serum and colostral (IgG, IgG1, IgG2) were higher purity. By using this purified IgG as a immunogen to immunize the rabbit, the polyclonal antibodies were characterized and applied to measure the serum and colostral IgG contents. The SDS-PAGE and western blot showed that the highest level of serum IgG was at 18 to 24 hr after birth .The serum IgG was the lowest level in the kids fed milk of late gestation. The results imply that the passive immunity or absorption of kid increases after colostrum feeding. The IgG concentration of jugular and mammary veins in dams showed biphasic patterns during 7day prepartum to 1 day postpartum and 3-7 day postpartum. At postpartum, the milk IgG level of dams showed a peak at parturition. At postpartum, the milk IgG level of dams showed a peak at parturition. At postpartum, the milk IgG level of dams was dramatically declined. The titer of anti-chicken RBC was not significant difference between kids fed colostrum, heat inactivated colostrum or milk of late gestation at 3 and 6 weeks old. These results suggest that the active immunity of kids may not be affected by the ammounts of Ig in feeding milk. The anti-chicken RBC titers were significantly higher in jugular vein and mammary secretes of cRBC-induced dam at day 1 postpartum was higher titer (P<0.05) of anti-chicken RBC than that non cRBC-induced dam. In addition, this trend was decreased at day 2 to day 7 postparturition. Comparing to the commercial bovine serum IgG1 and IgG2, the relative amounts of goat serum and colostral (IgG, IgG1, IgG2) were determined by sandwich enzyme link immunosorbent assay.