DEVELOPMENT OF APTAMER BASED CD62 DIAGNOSTIC KIT

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dc.contributor.advisor	Çevik, Özge
dc.contributor.author	AL-SAADI, MOHAMMED SATTAR ABDULJABBAR
dc.date.accessioned	2021-01-28T11:45:46Z
dc.date.available	2021-01-28T11:45:46Z
dc.date.issued	2021
dc.date.submitted	2020-12-23
dc.identifier.citation	Sattar M. Aydin Adnan Menderes University Health Science Institute, Molecular Biotechnology Programme, Master Thesis, Aydin, 2020	tr_TR
dc.identifier.uri	https://tez.yok.gov.tr/UlusalTezMerkezi/tezlerim.jsp?sira=0
dc.identifier.uri	http://hdl.handle.net/11607/3971
dc.description.abstract	Disease-specific biomarkers consider as important tool for the pathological conditions efficient management, including susceptibility determination, diagnosis, and preventive monitoring efficacy. P-selectin is selectively expressed after platelets activation, and it is involved in formation of thrombus, and also in immune response. It is known that serum and plasma p-selectin (CD62) levels increase in some pathological conditions such as heart attack, stroke, some immune diseases and cancer. To date, a lot of methods have been developed to measure p-selectin level. Aptamers use for targeting specific biomarkers on their molecular shape the basis. SELEX (The Systematic Evolution of Ligands by EXponential enrichment) is a process which uses to choose aptamers with high affinity for targeting specific macromolecular. In this study, a new aptamer-based kit was developed to measure CD62. Firstly, aptamers that specifically bind to CD62 were isolated using the SELEX method. Among the used aptamers, Apt-1, Apt-2 and Apt-3 were bound to CD62 protein with high affinity. The Apt-2, which binds with the highest affinity to CD62, the binding constant is -9,6 kcal/mol and dissociation constant (Kd) is 18.15±2.36 nM. We used Bovine serum albumin in the specificity test as a negative control and it was determined that there is no binding between the selected aptamers did not and this protein. The Intra and Inter assay performing showed that the average of Intra-assay was CV % 6,52 and the average of Inter-assay CV % 3,96. As a result, a sensitive, specific, time-saving and low cost kit was developed for the measurement of CD62 with this study.	tr_TR
dc.description.sponsorship	This project was supported by Aydin Adnan Menderes University Research Grant as a Graduate Research Project ADU-TPF-19051	tr_TR
dc.description.tableofcontents	LIST OF CONTENTS ACCEPTANCE AND APPROVAL PAGE …………..………………….………..… i ACKNOWLEDGEMENTS……………………………………………………...…… ii LIST OF CONTENTS………………………………………….………...…………... iii LIST OF ABBREVATĠONS……………..…………………….…………………….. vi LIST OF FIGURES………………………………………...………………………… viii LIST OF PICTURES…………………………………...…………………………….. ix LIST OF TABLES……………………………………………...…………………….. x ABSTRACT…………………………………………………………………………... xi ÖZET…………………………………………………………………………………. xii 1. INTRODUCTION…………………….…………….…… ……………………….. 1 1.1. Aptamers……………………..…………………………………………………... 1 1.1.1. Characteristics of Aptamers …………………………………………………… 2 1.1.2. Structure and Function of Aptamers………...…………………………………. 5 1.1.3. DNA and RNA Aptamers …………….……………………………………….. 6 1.1.4. Aptamer Differences with Monoclonal-Antibody………..…………………… 7 1.2. The SELEX………………………………………………….…………………… 10 1.2.1. The Principles of SELEX …………………….……………………………….. 10 1.2.2. Synthesis of ssDNA and RNA Aptamers ……….……………..……………… 10 1.2.3. Synthesis of Oligonucleotides Sequences Library …………………..………… 11 1.2.4. Aptamer Selecting and Enrichments …………………………..………………. 12 1.3. Aptamers Structure Modifications……………………………………………….. 14 1.4. The Selectins……………..………………………………………………………. 14 1.4.1. L-Selectin………………………………………………………………………. 17 1.4.2. P-Selectin………………………………….…………………………………… 18 1.4.3. E-Selectin………………………………………………….…………………… 18 iv 1.5. Platelets………………………………………...………………………………… 18 1.5.1. Platelets Activation…………………………………….………………………. 19 1.5.2. Platelets Activation Pathways……………………….…………………………. 19 1.6. Cellular Interactions……………………………………………………………… 20 1.7. Thrombosis…………………………….………………………………………… 20 1.8. Aptamer-Protein Interaction……………………………………..………………. 21 2. MATERIALS AND METHODS……………………….………………...…...…… 23 2.1. Materials…………………………………………………………………………. 23 2.1.1. Equipments…………………………………………………………………….. 23 2.1.2. Instruments…………………………………………………………………….. 23 2.1.3. Chemicals………………………………………………………………………. 24 2.2. Methods………………………………………………………………………….. 24 2.2.1. Building Aptamer by SELEX………………………………………………..… 24 2.2.2. Determination of Binding Affinity (KD)……………….……………………… 25 2.2.3. Direct ELONA TEST Protocol…………………………….………………….. 26 2.2.4. Western Blotting Protocol……………………………………………….…….. 27 2.2.4.1. BCA Protein Determination…………………………………………………. 27 2.2.4.2. Immunoblotting Assay………………………………………………………. 28 2.2.5. ELONA Kit Validation and Quality Testing…………………………………... 29 3. RESULTS…...………………………………………………….………………….. 30 3.1. Cell SELEX Studies …..………………………………………………………… 30 3.2. Aptamer Binding Affinity Characteristics ………………………………………. 32 3.3. ELONA Kit Validation and Quality Tests Results …..………………………….. 34 3.3.1. Sensitivity and Spesifity Tests…………………………………………………. 34 3.3.2. Intra and Inter Assay Tests Results…………………………………………….. 36 3.3.3. Recovery Tests Results………………………………………………………… 37 3.3.4. Linearity Test Results………………………………………………………….. 38 v 3.4. CD62 Detection Results in Real Human Sample………………………………... 38 4. DISCUSSION…..…………………………………………………………………. 40 5. CONCLUSION AND RECOMMENDATION………………………………….... 45 REFERENCES……………………………...……...………………………………… 46 CURRICULUM VITAE……………………………………………………………… 50	tr_TR
dc.language.iso	eng	tr_TR
dc.publisher	Adnan Menderes Üniversitesi, Sağlık Bilimleri Enstitüsü	tr_TR
dc.rights	info:eu-repo/semantics/openAccess	tr_TR
dc.subject	Aptamer, CD62 protein, p-selectin, ELONA, platelet	tr_TR
dc.title	DEVELOPMENT OF APTAMER BASED CD62 DIAGNOSTIC KIT	tr_TR
dc.type	masterThesis	tr_TR
dc.contributor.authorID	10376588	tr_TR
dc.contributor.department	Adnan Menderes Üniversitesi, Sağlık Bilimleri Enstitüsü, Moleküler Biyoteknoloji Anabilim Dalı	tr_TR