Dr. Thaweesak Tirawatnapong Chula Medical Research Center (Chula MRC)

Slides:

Advertisements

Similar presentations

Research Techniques Made Simple: Polymerase Chain Reaction

Advertisements

Nick Curry, MD, MPH Infectious Diseases Prevention Section

PCR, Gel Electrophoresis, and Southern Blotting

By Gracie Canales August 10, 2010

Global Consultation on the Implementation of the Xpert MTB/RIF system for rapid diagnosis of TB and MDR-TB M. Akhalaia, MD, Microbiologist, Reference.

Multiplex digital nucleic acid quantitation using molecular barcodes

Utilizing a Non-Commercial Real- Time PCR to Detect HIV-1 RNA in HIV Antibody Negative Diagnostic Sera Submitted to The Maryland Public Health Laboratory.

Pediatric Diagnosis of HIV-1 Infection Using Dried Blood Spots Chin-Yih Ou, PhD NCHSTP/DHAP Centers for Disease Control and Prevention.

The Current Pipeline for Point-of-Care Virologic Testing for HIV/AIDS Scaling up Virologic Diagnostic HIV Testing in Infants and Rationalizing Decentralization.

REAL TIME PCR ………A step forward in medicine

Simplification, cost-reduction strategies and examples from the field Teri Roberts Diagnostics Advisor Médecins Sans Frontières, Access Campaign 7th.

CFTR Genotyping Cutting Lab. When we receive blood from a study participant, we refrigerate it for 2-3 weeks which enables better DNA extraction from.

Nucleic Acid Extraction Control in Real-Time PCR Assays Steve Hawkins Senior Global Product Manager Bioline.

Chapter Six Nucleic Acid Hybridization: Principles & Applications 1.Preparation of nucleic acid probes: - DNA: from cell-based cloning or by PCR. Probe.

Molecular Testing and Clinical Diagnosis Amplified nucleic acid testing Part III.

Microarray Simultaneously determining the abundance of multiple(100s-10,000s) transcripts.

Class 6 DNA Arrays BIOMEMS, Fall Content u Polymerase Chain Reaction or PCR u DNA Detection Process u DNA Micro Arrays u Electronic DNA Arrays u.

Assays Molecular Diagnostics CSULA. What’s a molecular diagnostic assay? n A laboratory test for the presence or absence of a particular type of molecule.

New Molecular Based Methods of Diagnosis

RNA-Seq An alternative to microarray. Steps Grow cells or isolate tissue (brain, liver, muscle) Isolate total RNA Isolate mRNA from total RNA (poly.

1 Characterization, Amplification, Expression Screening of libraries Amplification of DNA (PCR) Analysis of DNA (Sequencing) Chemical Synthesis of DNA.

HCV Diagnostics Technology Landscape AIDS 2014, 10 th International AIDS Conference 21 July 2014 Maurine M. Murtagh UNITAID Consultant.

Genetic Technologies By: Brenda, Dale, John, and Brady.

Applied Biosystems 7900HT Fast Real-Time PCR System I. Real-time RT-PCR analysis of siRNA-induced knockdown in mammalian cells (Amit Berson, Mor Hanan.

Detection of Mutations in EGFR in Circulating Lung-Cancer Cells Colin Reisterer and Nick Swenson S. Maheswaran et al. The New England Journal of Medicine.

Basic Procedures for DNA analysis I) DNA isolation & purification: –Sample: nucleated cells –Principle: A- PURIFICATION STEPS: 1.Cell lysis 2.Removal of.

Genomic DNA purification

Laboratory Investigation

with an emphasis on DNA microarrays

 The HIV virus can mutate in HIV positive patients taking Anti-Retroviral Therapy (ART)  Their HIV strain has now become drug resistant (DR), and their.

COBAS AmpliPrep/Cobas TaqMan HIV-1 Test

APPLICATIONS OF MOLECULAR BIOLOGY TECHNIQUES TO MEDICAL MICROBIOLOGY.

Objective DNA amplification (eg. PCR)    advances in forensic, clinical applications Comparable protein amplification tools (?)  aid medical diagnostics,

BioLife Plasma Services Experience with HBV NAT Testing

Dr. Sumbul Fatma Department of Medical Biochemistry.

Recombinant DNA Technology……….. BTEC3301. DNA Libraries How do you identify the gene of interest and clone only the DNA sequence you are interested? Read.

Chapter 13: DNA Quantitation.  Quantitation determines the amount of human DNA present in an extract  A narrow concentration range is required to “seed”

Point of Care Testing – Clostridium difficle Amita Patel Guy’s and St Thomas’ NHS Foundation Trust.

Julia Robbins August 11, Objectives Clinical Significance of MRSA in Healthcare Setting Principle of assay Assay Procedure Assay Perfomance.

HCV PCR By Henrietta Orji July 31 st, 2010 Hepatitis C Virus by Polymerase Chain Reaction.

Nucleic Acid Purification : Its Principle and Miniaturization MEC seminar Apr. 13 Ji Youn Lee.

Molecular Techniques in Microbiology These include 9 techniques (1) Standard polymerase chain reaction Kary Mullis invented the PCR in 1983 (USA)Kary.

 DNA (gene mutations, paternity, organs compatibility for transplantations)  RNA  Proteins (gene expression)

LAB. DIAGNOSIS OF VIRUSES 5 methods are used for diagnosis in the virology laboratory: 1.Direct microscopy 2.Cultivation of viruses 3.Serology 4. Detection.

PHARMACOBIOTECHNOLOGY.  Recombinant DNA (rDNA) is constructed outside the living cell using enzymes called “restriction enzymes” to cut DNA at specific.

Molecular profiling of residual TNBC after neoadjuvant chemotherapy Yonsei Genomics Center Hanna Lee.

The Application of Real-Time PCR in the Diagnosis of Infectious Disease The Application of Real-Time PCR in the Diagnosis of Infectious Disease T.P.Sloots.

Molecular Testing and Clinical Diagnosis

A Nanoliter-Scale Nucleic Acid Processor with Parallel Architecture Jong Wook Hong, Vincent Studer, Giao Hang, W French Andreson, Stephen R Quake presented.

Chapter 10: Genetic Engineering- A Revolution in Molecular Biology.

目录 The Principle and Application of Common Used Techniques in Molecular Biology chapter 18.

Rapid Molecular Diagnostic Test of HIV-1 Purified RNA from Plasma Michael M. Ling, Ph.D

Virology – Diagnosis JU- 2 nd Year Medical Students By Dr Hamed AlZoubi – Microbiology and Immunology Department – Mutah University. MBBS (J.U.S.T) MSc,

PCR With PCR it is possible to amplify a single piece of DNA, or a very small number of pieces of DNA, over many cycles, generating millions of copies.

The Factor II (Prothrombin) G20210A Detection and Genotyping

Green with envy?? Jelly fish “GFP” Transformed vertebrates.

Lab-on-a-Chip The Ideal Technology for Bio-chemical Analysis

BioMérieux’s commitment in the fight against HIV Michel Bonnier VP Public Health.

Rajan sharma.  Polymerase chain reaction Is a in vitro method of enzymatic synthesis of specific DNA sequences.  This method was first time developed.

Viro-chip Microarray Using a Pan-Viral Microarray Assay (Viro-chip) to Screen Clinical Samples for Viral Pathogens.

Chapter 13: DNA Quantitation.  Determining the amount of DNA is a sample is essential  A narrow concentration range is required for PCR  Must use human-specific.

Midterm Review Feb

POLYMERASE CHAIN REACTION TECHNIQUES

A non-amplification molecular probe approach John Gerdes, Ph. D.

扩增产物的毛细管电泳分离 ( Amplification of capillary electrophoresis separation )

Crystal digital PCR for detection and quantification of circulating EGFR mutations in advanced non-small cell lung cancer Cécile Jovelet Postdocoral fellow.

Introduction to cDNA Microarray Technology

CHAPTER 12 DNA Technology and the Human Genome

CasE13a Schematic of the development of antibiotic resistance and how it can spread to humans.

Fig. 3 Single-molecule DNA recovery and amplification.

Presentation transcript:

Dr. Thaweesak Tirawatnapong Chula Medical Research Center (Chula MRC) New Technologies and Innovations in Laboratory Support of HIV/AIDS care and Treatment Dr. Thaweesak Tirawatnapong Chula Medical Research Center (Chula MRC)

Diagnostics Tests for HIV 1 Tests to facilitate initial diagnosis 2 Tests to stage the patients 3 Tests to monitor the patients

Important of HIV Testing Known HIV status for care and treatment For prevention measure Problem Poor HIV testing coverage in resource- limited Setting

General Community Requirement Need to increase the level of access to high quality diagnostic in resource-limited settings To facilitate early detection and treatment of HIV/AIDS Simplify and improve the efficiency of HIV testing Tests design to be delivered at The point of care (POC) or Near POC

The Various PCR Process have Three Steps in Common 1. Sample preparation, including viral concentration and nucleic acid extraction. 2. Amplification of the target DNA or RNA. 3. Detection of the amplified product.

DNA Extraction Flow with Magtration Technology

Automated Nucleic Acid Extraction

Extraction and PCR Set Up Qiagen Symphony Cobas Ampriprep

COBAS® S 201 System for Blood screening

Chiron Tigris for Blood screening

New Technologies for Viral Load Testing Alere NAT system disposable cartridge that provides for sample collection, cell lysis, specific target capture, reverse transcription, polymerase chain reaction amplification and real time fluorescence detection based on reporter probe hybridization on an integrated micro probe array.

Lab-in-a-tube Technology The Liat System automates all testing processes Sample preparation Amplification Real-time detection

Portable Fully Automate real-time PCR

The Liat™ Analyzer is developed for nucleic acid based testing and the Liat™ Tubes serve both as collection devices and as test chambers, maintaining samples in a closed system from sample collection through sample disposal. We believe that the Liat™ system is suitable for a wide range of testing labs and near-patient test settings due to its ease of use, fast turnaround time, cost effectiveness and safety features.

SAMBA: Simple AMplification Based Assay

Cepheid GeneXpert System

GeneXpert Cartridge and Module

Lab-on-Chip

Handy Lab

Microfluidic Technology

Nucleic acid extraction

QP system

BIST: Beads array In Single Tip

New HIV Drug resistant testing Minisequencing or Single base extension

Bio-Strands Technology

Nanostring Technology

Hybridization NanoString’s Technology employs two ~50 base probes per mRNA that hybridize in solution. The Reporter Probe carries the signal; the Capture Probe allows the complex to be immobilized for data collection

Purification and Immobilization After hybridization, the excess probes are removed and the probe/target complexes aligned and immobilized in the nCounter Cartridge.

Data Collection Sample Cartridges are placed in the Digital Analyzer for data collection. Color codes on the surface of the cartridge are counted and tabulated for each target molecule

nCounter Analysis System High level of precision High level of sensitivity (<1 copy per cell) No enzyme processing or Amplification Quantification

Multiplexed Diagnostic LLNL Awarded $2.5M to Move Pathogen Detection Tests to NanoString Platform June 07, 2011 The National Institutes of Health has awarded $2.5 million to researchers at Lawrence Livermore National Laboratory to support the development of pathogen detection assays on NanoString Technologies' nCounter system. The project aims to develop high-content, multiplex assays capable of simultaneously detecting 35 National Institute of Allergy and Infectious Diseases category A, B, and C viral agents, plus quantifying cytokine and chemokine responses in patients,

Science 24 June 2011: Vol. 332 no. 6037 p. 1497 BIOTECHNOLOGY Lab-on-a-Chip Maker Looks to Put Hong Kong on Biotech Map

RMD Automation Strategy - Maximize Testing Efficiency Reduce complexity and increase automation, throughput Complexity Today Near-Term Long-Term Virology & Blood Screening Amplicor LC 2.0 CAP/CTM & cobas s 201 cobas s 401 cobas Amplicor COBAS® TaqMan® 48 Other (HPV, CT/NG, Micro/Oncology) CAP/CTM 96/48 & cobas s 201 New Generation systems cobas 4800 cobas s 401

Thank you