1 / 45

Preanalytical Errors in Medical Laboratories

Preanalytical Errors in Medical Laboratories. Ashishkumar Soni QMS Manager – West Randox Laboratories India Pvt. Ltd. Objectives. Identify the significant pre-analytical errors that can occur during blood specimen collection and transport

mora
Télécharger la présentation

Preanalytical Errors in Medical Laboratories

An Image/Link below is provided (as is) to download presentation Download Policy: Content on the Website is provided to you AS IS for your information and personal use and may not be sold / licensed / shared on other websites without getting consent from its author. Content is provided to you AS IS for your information and personal use only. Download presentation by click this link. While downloading, if for some reason you are not able to download a presentation, the publisher may have deleted the file from their server. During download, if you can't get a presentation, the file might be deleted by the publisher.

E N D

Presentation Transcript

  1. Preanalytical Errors in Medical Laboratories Ashishkumar Soni QMS Manager – West Randox Laboratories India Pvt. Ltd.

  2. Objectives • Identify the significant pre-analytical errors that can occur during blood specimen collection and transport • Explain the various means of pre-analytical error prevention • List proactive steps to reduce potential pre-analytical errors associated with blood collection and transport

  3. Total Quality Laboratory Quality means achieving positive patient outcomes through control of pre-analytical, analytical, and post-analytical error.

  4. There are a variety of potential errors that can affect the quality of the laboratory results. • Pre-analytical errors • Before the sample reaches the laboratory • Analytical errors • During the analysis of the sample • Post-analytical errors • Occurring after the analysis

  5. Introduction • Three phases of laboratory testing: Pre-analytical, Analytical and Post-analytical Now termed as Pre Examination,Examination & Post Examination (As per ISO 15189) • Pre-analytical : Test order by clinician, Instruction to the patients, Specimen collection, Storage, Transport and processing (for eg. Centrifugation) • Analytical : Testing • Post-analytical : Retesting- if required, Results Transmission, Interpretation, follow-up,.

  6. Pre-analytical errors • Pre- and post-analytical errors are estimated to constitute 90% of errors • Errors at any stage of the collection, testing and reporting process can potentially lead to a serious patient misdiagnosis • Errors during the collection process are certainly inevitable and can be prevented with a diligent application of quality control, continuing education and effective collection systems

  7. Types of Preanalytical Errors • Patient Identification • Phlebotomy Technique • Collection Procedures • Specimen Transport • Specimen Processing

  8. Pre - Analytical Errors…Before the sample reaches the laboratory but directly affect the quality and clinical usefulness of the final result. Improper preparation of the patient:- • patient fasting • glucose test • stress and anxiety • urinary protein

  9. Pre - Analytical Errors… • Improper preparation of the patient • Improper collection of the blood sample:- • sample haemolysis • LDH, potassium or inorganic phosphate • insufficient sample volume • unable to carry out all requested tests • collection timing • 24 hour urine

  10. Pre - Analytical Errors… • Improper preparation of the patient • Improper collection of the blood sample • Incorrect specimen container:- • serum or plasma • fluoride tubes for glucose • to inhibit glycolysis • EDTA unsuitable anti-coagulant for calcium

  11. Pre - Analytical Errors… • Improper preparation of the patient • Improper collection of the blood sample • Incorrect specimen container • Incorrect specimen storage:- • sample left overnight at room temperature • falsely elevated K, Phos and red cell enzymes • delay in sample delivery • falsely lowered levels of unstable analyte (NEFA)

  12. The sex of the patient male or female The age of the patient new born / juvenile / adult / geriatric Dietary effects low carbohydrate / fat high protein / fat When the sample was taken early morning urine collection pregnancy testing Patient posture urinary protein in bed-ridden patients Other Factors…

  13. Effects of exercise creatine kinase / CRP Medical history heart disease / diabetes / existing medication Pregnancy hormonal effects Effects of drugs and alcohol liver enzymes / dehydration Other Factors…

  14. Patient Identification Errors in correctly identifying the patient are indefensible • Reasons for patient identification errors : • Patient identification from identification bracelet (inpatients) • Proper positive patient identification procedures not followed • Patient identification by asking patients to state or spell their full name (inpatients/outpatients) • Patient identification by staff or family member if patient unable to identify him/herself

  15. Patient Identification Specimen tubes unlabeled Requisition or collection tube labels not affixed to tubes • Requisition or collection tube labels in bag containing collection tubes • Requisition or collection tube labels rubber-banded to tubes • Collection tube labels not affixed to all tubes • Specimen collection tubes labeled insufficiently with at minimum patient’s full name, date/time of collection, phlebotomist’s initials

  16. Patient Identification Collection tubes labeled with the wrong patient • Wrong computerized labels affixed to collection tubes at bedside • Collection tubes not labeled at the time of collection • Collection tubes incorrectly labeled by someone other than the phlebotomist who collects the specimen

  17. Phlebotomy Errors • Phlebotomy is a highly complex skill requiring expert knowledge, dexterity and critical judgment • Phlebotomy errors may cause harm to patients (For eg. Thrombosis) or result in needle-stick injury to the phlebotomist

  18. Phlebotomy Technique • Phlebotomy technique is important • Ensures test result validity • Minimizes trauma to patient • Minimizes potential for phlebotomist injury • Reduces recollections • Vein selection essential for successful venipuncture • Three veins in antecubital fossa in order of selection (1) median cubital (2) cephalic (3) basilic

  19. Venipuncture site selection • Although the larger and fuller median cubitalvein of the arm is used most frequently, cephalic and basilic veins are also acceptable for venipuncture.

  20. Phlebotomy Technique • Site Selection • Use alternative arm or draw below IV to avoid contamination/dilution from IV • Avoid sites with IV • Document arm if IV • Mastectomy—avoid site due to lymphostasis • Infection risk/alteration in body fluids and blood analytes • Edematous areas —avoid due to accumulation of body fluids • Possible contamination/dilution of specimen

  21. Phlebotomy Technique • Venous Access Difficulties • Obstructed, hardened, scarred veins • Veins difficult to locate • Use of Alternative sites • Top of hand/Side of wrist • Areas to avoid • Vein Collapse • Use of appropriate needle size • Smaller evacuated collection tube

  22. Phlebotomy Technique • Tourniquet Application • Tourniquet tied too close to the venipuncture site can cause hematoma • Veins may not become prominent if tourniquet is tied too high (more than 3 to 4 inches above venipuncture site) • Tourniquet left on longer than one minute can result in hemoconcentration, affecting some test results • Tourniquet should be released as soon as needle is in the lumen of the vein and blood flow established

  23. Phlebotomy Technique • Cleansing of venipuncture site • Thorough cleaning with alcohol • Allow alcohol to dry completely to avoid stinging sensation upon needle entry and hemolysis of sample • Samples such as blood cultures should be collected using iodine to cleanse site to ensure sterility of sample • Recollection rate for blood cultures ranges due to contamination is as high as 50% in hospitals with increased costs, patient overtreatment

  24. Phlebotomy Technique • Correct collection system • Evacuated tube system (Vacutainer) for large veins in antecubital fossa • Syringe for small, fragile veins or veins outside antecubital fossa • Venous access • Needle entry should be at 15 to 30 degrees angle depending on depth of vein • Needle entry should be in same direction as vein, centered over vein • Anchor vein to prevent movement during needle entry and to reduce pain to patient

  25. Collection Procedures • Order of Draw • Order of draw affects the quality of the sample and can lead to erroneous test results due to contamination with the additive from the previous blood collection tube • Hemolysis • Blood collected insufficient to amount of additive in tube (Ratio of anticoagulant to Blood) • Traumatic venipuncture • Blood collected from area with hematoma • Vigorous shaking of tubes after collection • Milking the site when collecting capillary samples and blood collected using a small diameter needle.

  26. Order of Draw for Multiple Tube Collections • 1. Blood culture containers • 2. Blue top tubes • 3. Red top tubes • 4. Green top tubes • 5. Lavender top tubes • 6. Gray top tubes

  27. Red • No anticoagulant present • Tests using serum which include: most blood chemistries, serology tests.

  28. Light Blue • Additive - Sodium Citrate • Tests: Coagulation studies - PT, PTT, fibrinogen, etc. • MUST BE FILLED COMPLETELY.

  29. Lavender Top Tube • Additive =EDTA (Ethylene Diamine Tetra Acetic Acid) • Hematology

  30. Green • Sodium heparin, lithium heparin or ammonium heparin. • STAT blood chemistries.

  31. Gray • Additive: • Potassium oxalate and sodium fluoride. • or Na2 EDTA and sodium fluoride. • Glucose.

  32. Blood Cultures • Not for routine laboratory analysis, special collection to detect bacteria growing in blood. • Site preparation VERY important.

  33. Collection Procedures • Timing of Collection • Timed Draws • Therapeutic Drug Monitoring • Peak and trough collection times • Basal State Collections • Fasting requirements—no food or liquid except water • Specimens affected by time of day, for example, cortisol

  34. Collection Procedures • Improper collection tube drawn for test ordered Example - No gel tubes should be used for collection of drugs testing • Collection tube not completely fille • Example—light blue top tube for Coagulation Studies. Incomplete filling results in specimen dilution and erroneous Prothrombin and aPTT test results.

  35. Collection Procedures • Capillary Collections (Finger stick or heel stick) • Appropriate site • Heel stick—sides of the bottom surface of the heel • Finger stick—third or fourth fingers, perpendicular to fingerprint lines on fleshy pads on finger surface • Warm before collection to increase capillary blood flow near skin surface • Cleanse site with alcohol and allow to air dry

  36. Collection Procedures Capillary Collections • Massaging site to increase blood flow • Milking site can cause hemolysis or tissue fluid contamination • Finger sticks—roll fingers toward fingertip at 1st finger joint several times • Heel sticks—gently squeeze infant’s heel before performing puncture. • Perform puncture while firmly squeezing finger or heel • Wipe away first two drops of blood • Ensure that full blood drop wells up each time

  37. Collection Procedures Capillary Collections • Avoid touching capillary collection tube or micro collection tube to skin or scraping skin surface • Contaminates puncture site • Blood may become hemolyzed • Mixing micro collection tubes with additive frequently to avoid micro clots • Collecting tubes with additives first • Protecting tubes for bilirubin from light

  38. Transportation Transport of blood specimens in the proper manner after collection ensures the quality of the sample • Timing • Some specimens must be transported immediately after collection, for example Arterial Blood Gases. • Plasma for coagulation tests must be seperated within 30 mins of collection • Specimens for serum or plasma chemistry testing should be centrifuged and separated within two hours

  39. Transportation • Temperature • Specimens must be transported at the appropriate temperature for the required test • On ice—ABGs, Ammonia • Warmed -98.6 degrees (37 C) for cryoglobulins • Avoid temperature extremes if transported from via vehicle from other collection site • Transport Container • Some samples need to be protected from light, for example, bilirubin • Transport in leak-proof plastic bags in lockable rigid containers

  40. Processing • Centrifugation Right speed & time very imp to avoid hemolysis • Storage Even after testing is done, many times samples are required for rechecks, or test edition / addition • Pre-treatment of Samples Required for tests like HbA1c, G6PD etc Best procedure is to follow manufacturer’s guidelines

  41. Error Prevention • Phlebotomy Education • Phlebotomists should have completed a standard academic course in phlebotomy and undergo thorough on-the-job training under the supervision of a senior phlebotomist • Continuing Education • Phlebotomists should participate in regular educational competency assessments (written and observational) • Phlebotomy resources • Adequate staffing to maintain collection standards • Use of vaccutainers & barcodes

  42. Conclusion • Good quality assurance vital for the laboratory to reduce errors and ensure confidence in patient results • Implementation of a good laboratory quality assurance package, while appearing to represent additional costs to the lab’s budget will in the long run: • Decrease lab cost by eliminating need to run unnecessary additional tests! • Decreased cost of running entire hospital by preventing inappropriate patient care!

  43. Let’s Discuss • How are pre-analytical errors prevented in your laboratory? • What technology do you use to prevent human error? • What systems does your laboratory use to prevent errors by non-laboratory staff collecting blood? • What pro-active improvements would reduce the number of pre-analytical errors?

  44. Thank you for your Kind Attention Golden Rule of Clinical Laboratory Science “No result is better than a wrong result.”

More Related