Blood Collection and Processing SOP



Similar documents
Standard Operating Procedure (SOP) Work Package 8. Sample Collection and Storage

Laboratory Biosafty In Molecular Biology and its levels

LAB 11 PLASMID DNA MINIPREP

HARVESTING AND CRYOPRESERVATION OF HUMAN EMBRYONIC STEM CELLS (hescs)

Archived. Gloves should be changed frequently during the analysis.

Biosafety Level 2 (BSL-2) Safety Guidelines

DNA Analyst Training Laboratory Training Manual Protocol 2.02 Clean Technique

Olympic B3 Summer Science Camp 2015 Weller, Smith, Putnam L3

INMA LABORATORY MANUAL

PEAC CENTRAL LABORATORY SAMPLING MANUAL

Agencourt RNAdvance Blood Kit for Free Circulating DNA and mirna/rna Isolation from μL of Plasma and Serum

GENOME RUSSIA PROJECT BLOOD SAMPLES COLLECTION, DNA EXTRACTION AND DNA QUALITY CONTROL PROTOCOLS

NimbleGen DNA Methylation Microarrays and Services

Procedure for RNA isolation from human muscle or fat

UltraClean PCR Clean-Up Kit

DNA SPOOLING 1 ISOLATION OF DNA FROM ONION

Protocol Micro Lab. K:\Microlab_protocols\Protocols_active\03 Instrument manuals\ml03_001_001 DGGE.doc. Preparation of gels

UltraClean Soil DNA Isolation Kit

Quantifying Bacterial Concentration using a Calibrated Growth Curve

School of Chemistry and Chemical Biology Hazardous Waste Management Plan

RealLine HCV PCR Qualitative - Uni-Format

Plant Genomic DNA Extraction using CTAB

Gentra Puregene Handbook

KGI MEDICAL WASTE MANAGEMENT PLAN

Biosafety Spill Response Guide

RNA Extraction and Quantification, Reverse Transcription, and Real-time PCR (q-pcr)

UNIVERSITY OF RICHMOND REGULATED MEDICAL WASTE MANAGEMENT GUIDELINES

Chromatin Immunoprecipitation (ChIP)

Infectious Waste Management Plan

INTRODUCTION. Viral shedding is crucial for Gene Therapy Products Safety linked with shedding data

Transformation Protocol

Scott & White Institutional Biosafety Committee Compliance Program Biohazardous Material Spill Clean-Up Procedure Policy #IBC.002

Protocol for Disinfection of Cell Culture and Tissue Culture in Media:

Parent & Healthcare Professional Instructions for the collection of Maternal & Umbilical Cord Blood

Policies. Prep Room Policies

HANDLING OF RADIOACTIVE WASTES

Protein expression in the life cycle of bean beetles (Callosobruchus maculatus)

AxyPrep Blood Genomic DNA Maxiprep Kit

Lab Safety and Standard Operating Procedures. Faculty of Dentistry And School of Biomedical Engineering

Revised EHS Biosafety. 1 Select appropriate containers/bags for autoclaving.

Introduction BIOMEDICAL WASTE

Biohazardous Waste Disposal. Table of Contents

Please note: Contact Coppe Laboratories at if archival plasma samples need to be tested.

Kevin Bogart and Justen Andrews. Extraction of Total RNA from Drosophila. CGB Technical Report doi: /cgbtr

Biohazardous, Medical & Biological Waste Guidance Chart

Human Peripheral Blood Mononuclear Cell (PBMC) Manual

Appendix J IBC Biohazard Spill Management Plan

Guidelines for Ethidium Bromide Waste Management & Disposal. University of Tennessee-Knoxville

QIAGEN Supplementary Protocol

LABORATORY WASTE DISPOSAL GUIDELINES

STA DARD OPERATI G PROCEDURE FOR THE DETECTIO OF AFRICA SWI E FEVER VIRUS (ASFV) BY CO VE TIO AL POLYMERASE CHAI REACTIO (PCR)

Detailed protocol: Combined method for RNA isolation. from cartilage

Coating and Extraction of Honeycomb Denuders

Beware that ordinary prescription glasses do not provide adequate protection. This is also true with poorly fitting safety glasses.

Fundamental Autoclave Techniques

OCCUPATIONAL SAFETY AND ENVIRONMENTAL HEALTH GUIDELINE

PCR and Sequencing Reaction Clean-Up Kit (Magnetic Bead System) 50 preps Product #60200

Blood sampling and transportation Standard Operating Procedure

Sanger Sequencing: Sample Preparation Guide

Response to Biological Spills in the Laboratory (Intentional or Accidental)

VACUETTE RNAgard Blood Tubes BioMaxi Blood RNA Purification Kit. For the collection, preservation and purification of RNA from whole blood

Assessment of Islet Functional Potency by Glucose Stimulated Insulin Secretion

Central Line Blood Draw

DNA Isolation Kit for Cells and Tissues

ELUTION OF DNA FROM AGAROSE GELS

Appendix H IBC Managing Biohazardous Waste SOP

Optimal management of RA patients who require Biologic Therapy. (ORBIT Study) SAMPLING MANUAL

RADIATION CONTROL TECHNIQUE #2 INSTRUCTIONS FOR PREPARATION OF RADIOACTIVE WASTE FOR DISPOSAL

THE UNIVERSITY OF NEWCASTLE- SCHOOL of BIOMEDICAL SCIENCES

Epinephrine/Norepinephrine ELISA Kit

GRS Plasmid Purification Kit Transfection Grade GK (2 MaxiPreps)

STANDARD OPERATING PROCEDURES SPILL RESPONSE AND CLEAN-UP OUTSIDE BIOSAFETY CABINET

ENVIRONMENTAL HEALTH, SAFETY & RISK MANAGEMENT. Hazardous Materials &Waste Management Plan at

CatCombi Research ELISA Kit

Decontamination and Waste Management

Appendix H Managing Biohazardous Waste SOP

The fastest spin-column based procedure for purifying up to 10 mg of ultra-pure endotoxin-free transfection-grade plasmid DNA.

Inc. Wuhan. Quantity Pre-coated, ready to use 96-well strip plate 1 Plate sealer for 96 wells 4 Standard (liquid) 2

INSTITUTIONAL POLICY AND PROCEDURE (IPP)

PowerFecal DNA Isolation Kit

Aseptic Technique. A GMP/GTP Training Module

Contents. XI. Materials and Equipment Needed But Not Provided 5. DNA Extraction from Small Amount of Tissue 10

A Guide to Managing Your Biological Waste at the University at Albany

Classic Immunoprecipitation

UltraClean Forensic DNA Isolation Kit (Single Prep Format)

One Shot TOP10 Competent Cells

MasterPure RNA Purification Kit

AUTOCLAVE PROGRAM. SOP Bio-006 FOR THE USE OF AUTOCLAVE FOR STERILIZATION OF MATERIALS AND BIOLOGICAL WASTE SOP

Dot Blot Analysis. Teacher s Guidebook. (Cat. # BE 502) think proteins! think G-Biosciences

Southern Blot Analysis (from Baker lab, university of Florida)

Mouse krebs von den lungen 6 (KL-6) ELISA

Mouse Creatine Kinase MB isoenzyme (CKMB) ELISA

Mouse Keyhole Limpet Hemocyanin antibody(igm) ELISA Kit

Transformation Kit BACTERIAL TRANSFORMATION: GREEN FLUORESCENT PROTEIN. Partnership for Biotechnology and Genomics Education

Policy for the Disposal of Biological Waste

Dartmouth College. Institutional Biosafety Committee. Biohazardous Waste Disposal Guide IBC Approved: 10/7/15

HiPer Total RNA Extraction Teaching Kit

QuickZyme Soluble Collagen Assay

RiboZol RNA Extraction Reagents

Transcription:

Brisbane Breast Bank Blood Collection and Processing SOP Breast Pathology Laboratory University of Queensland Centre for Clinical Research

Blood Collection We collect 30ml of blood from patients who have consented to take part in the study. Blood is collected in two EDTA tubes (10ml) and one plain tube (10ml). Blood is collected and placed on ice before transportation to the Breast Pathology Laboratory. Blood Processing Overview Log the sample in the tissue bank log book and provide the sample with the next consecutive blood number (B#) to de-identify the sample. The following aliquots are required: 1 x Guthrie Card 3 x Plasma (clear cap) aliquots 3 x Serum (yellow cap) aliquots 1 x Buffy coat (clear cap) aliquots 5 x Whole blood (clear cap) aliquots Blood Tubes Aliquots First purple cap 10ml EDTA tube Plasma in three 1.8ml clear capped tubes. Buffy coat in one 1.8ml clear capped tube. Second purple cap 10ml EDTA tube Guthrie card Whole blood in five 1.8ml clear capped tubes. Red cap 10ml plain Tube Serum in three 1.8ml yellow capped tubes. Brisbane Breast Bank (updated 13/09/2012) Page 2

Safety Procedures Treat all blood samples as potentially infections. Wear personal protective equipment (PPE) at all times: lab coat, safety glasses and double gloves. All processing of unscreened blood is to be performed in the biohazard in room 620. All non-liquid waste is to be double bagged and sealed. Liquid blood waste is discarded in blood waste containers that contain biodyne. Use two layers of bench coat. Materials Required for Blood Processing All materials required for processing can be found in the drawers near the biohazard hood. Place all items (tubes, racks, pipettes etc.) to be used into the hood BEFORE YOU BEGIN. List of items to be placed inside the hood (per patient): Two sets of bench coats 50ml tube (1) on a rack Sterile pasteur pipettes with bulb - one pack 1.8mL Tubes: yellow (3) and clear (9) in tube rack (label the tubes before starting or label during the centrifugation steps) Guthrie card (1) Blood waste container containing ~10mL biodyne a set of double-lined plastic bags 1X TE buffer Rack for the original blood tubes Items to place next to the hood: 70% ethanol and cavicide for cleaning the hood esky with ice tissues and paper towel gloves Brisbane Breast Bank (updated 13/09/2012) Page 3

Occasionally, there is less than 10ml of blood in the blood tubes. In this case, use the EDTA tube with the largest volume for whole blood aliquots and guthrie card. We prioritise whole blood over plasma aliquots. Process the EDTA tube for plasma first since plasma should be frozen quickly to preserve protein integrity. EDTA tubes (purple cap) First EDTA tube is for Plasma and Buffy coat Centrifuge at 3000rpm (1500g) for 10min. Handle with care as shaking disturbs the fractions. Plasma BC RBC For Plasma (P): Plasma fraction is the top layer after centrifuging Aliquot into 3 clear capped tubes labelled with the B# (lid and side of tubes), date and aliquot number (P1, P2 & P3) on the side of the tubes. Store at -80 in the plasma box. Record number of aliquots and any other details i.e. Green, cloudy etc. in the tissue bank log book. Record the location of the tubes on the plasma map sheet. For Buffy Coat (BC): This is the middle layer and is a white colour. Using a sterile pasteur pipette remove this layer into a 50ml tube containing approximately 50mls of 1x TE. Spin at 3000rpm (1500g) for 10min. Carefully pour off the supernatant into the blood waste container with biodyne, taking care that the pellet does not dislodge. Repeat this TE wash and spin. Carefully pour off the supernatant into the blood waste container with biodyne, taking care that the pellet does not dislodge leaving about 1ml of TE buffer. Transfer the pellet with 1ml of TE into a 1.8ml clear capped tube labelled with the B# (lid and side of tube), date and BC on the side of the tube. If the buffy coat is very red you will need to do the 1 x TE wash one more time. Brisbane Breast Bank (updated 13/09/2012) Page 4

Record number of aliquots and any other details in the tissue bank log book. Store BC in -80 freezer in BC box and record the location of the tube on the paper map sheet. Second EDTA tube is for whole blood aliquots and Guthrie card Do not spin this tube You can process this tube during the centrifugation steps of the first tube. For Guthrie Card The purpose for the Guthrie card is for quality assurance. If there is a concern that there may have been an error then the DNA can easily be extracted from the Guthrie card and cross referenced with the existing DNA. All blood processed requires a Guthrie card. It makes no difference if the patient has given a previous blood sample. Label the card with the B# and the date. Invert the second EDTA tube to ensure that the blood is mixed and then dot the card across one line (six dots in total). Allow the Guthrie card to dry overnight in the biohazard hood. Store the dried guthrie cards in the guthrie card storage box at room temperature in numeric order. For Whole Blood Aliquot blood into five 1.8ml clear capped tubes labelled with B# (lid and side of tubes), date and aliquot number (B1, B2, B3, B4 & B5) on the side of the tubes. Store at -80 in the blood box. Record number of aliquots and any other details in the tissue bank log book. Record the location of the tubes on the blood map sheet. Plain Tube (red cap) For Serum (S) Centrifuge at 3000rpm (1500g) for 10min. Serum fraction is the top layer after centrifuging. Aliquot the serum into 3 X 1.8ml tubes with a yellow cap labelled with B# (lid and side of tubes), date and aliquot number (S1, S2 & S3). Record number of aliquots and any other details i.e. Green, cloudy etc. in the tissue bank log book. Record location on the serum map sheet. Store at -80 in the serum box. Brisbane Breast Bank (updated 13/09/2012) Page 5

Cleaning up Spray pipettes, bottles etc with 70% ethanol when they come out of the biohazard hood. Spray centrifuge with 70% ethanol after use. Throw out the bench-coat into the double-bagged blood solid waste (containing blood tubes etc). Tie the double-bagged solid waste with autoclave tape and place it in the yellow-lined biological waste bin. Use cavicide to wipe the biohazard hood, rinse with water, then spray with 70% ethanol and wipe again. Press down arrow on the hood to turn the shield down. Then turn the hood off. Blood DNA Extractions DNA extractions from whole blood aliquot tubes are only done if the samples are requested for research projects. Extract the DNA using the Qiagen QIAmp Midi Blood Extraction Kit. Quantify the DNA using Nano drop and also check integrity of the DNA on a 1.5% agarose gel. Record the storage and concentration information in the tissue bank database. Store at -80 in the blood DNA box and record the map location. Solutions for Blood Processing 1X TE To prepare 1L of 1 X TE, add 10ml of 1M Tris HCl ph8.0 and 2mL of 0.5M EDTA ph 8.0, then make it up to 1L with milliq water. Brisbane Breast Bank (updated 13/09/2012) Page 6

2026 © DocPlayer.net Privacy Policy | Terms of Service | Feedback  | Do Not Sell My Personal Information