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Correlation Testing in Blood Bank
John C. Staley and 2 others reacted to Cliff for a topic
This is a good solution, I would like to suggest that you do not retest them until after the due date, not just the date you reported them.3 points -
Backtype discrepancy.. is it anti-a1?
Bet'naSBB and one other reacted to Melanie Oliveira for a topic
Sounds like ABO discrepancy due to a cold agglutinin which may or may not have specificity. I would run 3 M+ cells and 3 M neg cells at IS, RT and 4'C along with an autocontrol. IF only the M+ cells react at IS or RT, then I would ficin treat the A1 and B cells and repeat the reverse grouping using ficin treated cells. Just a suggestion.2 points -
positive dat w cord blood
Bet'naSBB and one other reacted to Malcolm Needs for a topic
Oh it is!!!!!!!!!!!!!!!!!2 points -
positive dat w cord blood
exlimey and one other reacted to Malcolm Needs for a topic
Do you think somebody should tell them that ABO HDFN sometimes gives a Negative DAT result in the fist two or three days of life, and that they might actually be better off looking for clinical signs, rather than performing diagnoses on the result of pathology results???????2 points -
positive dat w cord blood
exlimey and one other reacted to Malcolm Needs for a topic
I think that it depends upon the state of the baby. For example, if the mother is D Negative, and has been in receipt of anti-D immunoglobulin, and the baby has a positive DAT, but is showing no other signs of HDFN, then we wouldn't perform any further testing. If the baby has a lowish Hb, and the mother is group O and the baby group A or B, we may take a look at the mother's IgG ABO status, and then perform an eluate on the baby. Where we might really "go to town" is if the baby is showing overt signs of HDFN, we might well go the "whole hog" and perform an elution, just in case there is a maternal alloantibody directed against a low prevalence antigen also expressed on the red cells of the father. If this is suspected, it would be easy enough to adsorb out any IgG anti-A or anti-B on the baby's red cells, without adsorbing out the potential antigen against a paternal low prevalence antigen. The specificity of such an antibody would be interesting, but not necessarily vital, as, should the baby require a transfusion, suitable blood should be easy to obtain.2 points -
It is standard 5.1.2.4: The laboratory shall evaluate the comparability of test results obtained using different methods, instruments and if applicable testing sites. This shall be performed twice annually. We use old CAP samples or known patient samples with antibodies. Test them on the analyzer and with PEG on the bench.2 points
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We use our "old" CAP samples........... Once they've been turned in and reported, we assign them to techs using our "other" methods. SOP is gel/Ortho Vision Max Additional testing then would be manual gel, Peg, LISS, Saline. Same for titers and DAT's Seems to work pretty well for us!2 points
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Case study book
SbbPerson and one other reacted to Malcolm Needs for a topic
Thanks Lorna. I'll have a look and see what I can provide but, as I see that you are working in the Isle of Man, may I suggest you get a copy of the BCSH Guideline "Pre-Transfusion Compatibility Procedures in Blood Transfusion Laboratories" from 2012 (which is available free on-line - just put in BCSH Guidelines), and these have a few at the end of the Guideline. In addition, have a look on this site under "Library" at the top of the page, where you might find more than one thing (probably under "Education", but not only there), that will be of use to you.2 points -
This a classic case of Sensitivity vs Specificity. Clinical assays (including those in the transfusion medicine arena) are often designed to be as sensitive as possible, especially those intended to be frontline screens. Nobody wants to miss anything. However, the downside of this approach is that sometimes specificity suffers - more positives are obtained than desired. Solid Phase, Gel and PEG assays are super-sensitive, but may detect "nuisance" antibodies like weaker autoantibodies (warm and cold), or things like anti-P1, anti-Leb, or "HTLA-like" antibodies. Less sensitive assays that employ no enhancement (saline) or thing like LISS are sometimes used strategically to avoid the nuisances. Many institutions have policies that allow the deliberate down-regulation of sensitivity to ameliorate such problems. For example, performing crossmatches in LISS rather than Gel. Certainly, there's a risk that something might be missed using a less sensitive assay, but I think it's important to realize that in years past, the use of those less sensitive assays didn't leave a trail of bodies. In patients with long-term autoantibodies, it's not unusual for the autologous cells (DAT/autocontrol) to react weaker than Screening Cells or panel cells. The appears to be some kind of weakening of native antigens to which the autoantibody is directed. Sometimes, that may even mean the DAT is negative, but still yields a reactive eluate .2 points
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General Lab: Immunoglobulin
Cliff reacted to Malcolm Needs for a topic
I just answered this question. My Score PASS YEE- HAH!!!!!!! I got one right!1 point -
I just answered this question. My Score FAIL1 point
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BloodBankTalk: Largest blood donation event
Cliff reacted to Malcolm Needs for a topic
I just answered this question. My Score FAIL1 point -
Using platelets returned in a cooler with ice
John C. Staley reacted to Neil Blumberg for a topic
There is no evidence that cold stored platelets returned to room temperature need any change in outdating. I wouldn't go beyond 7 days for pathogen reduced platelets or 5 days for non-PRT platelets. Would just use clinical judgement. The reference above relates only to frozen platelets in any case, an entirely different critter, so not necessarily informative.1 point -
New QC manufacturer for blood bank automated analyzer
John C. Staley reacted to Cliff for a topic
I always start with the manufacturer. They will often provide suggested plans that you can then modify.1 point -
Happy Thanksgiving to all of our Canadian Pathlabtalk members1 point
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Correlation Testing in Blood Bank
Yanxia reacted to Mabel Adams for a topic
I feel like I saw that AABB added a standard that requires us to do correlation testing twice per year between antibody screening methods. Can anyone tell me which standard it is? I would also love to hear what you do for this standard when we expect Saline, Gel, PEG etc. to react differently and use those differences to avoid weak warm autos etc.1 point -
yes, that's what we wait for...........and we usually get behind and don't end up handing them out until we've already received the results.1 point
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Correlation Testing in Blood Bank
John C. Staley reacted to Mabel Adams for a topic
Can anyone explain the value of this effort to me? How do you change your tests if your results don't agree? (In Chemistry you probably recalibrate.) Do you just sign off when it is expected due to different sensitivity?1 point -
Correlation Testing in Blood Bank
Mabel Adams reacted to sgoertzen for a topic
Here is the form that we use. You need to have something written in policy that accounts for the expected variability of reactions when comparing different methods. We have multiple methods for ABO/Rh, Antibody Screen, Antigen Typing, Antibody ID, and AHG Crossmatch, so we have to do method comparison on all of these. TQ-0530F03 Method Comparison__blank_copy_id_10835032.pdf1 point -
Correlation Testing in Blood Bank
Mabel Adams reacted to Cliff for a topic
I don't have access to Standards anymore (I'm retired), and I don't recall if AABB requires them. The Joint Commission definitely does, and it asked for our 6-month correlations during every inspection.1 point -
Correlation Testing in Blood Bank
Mabel Adams reacted to Kelly Guenthner for a topic
Our "methods" are automated gel, manual gel & tube (PEG). We do not evaluate our alternate enhancements as different "methods".1 point -
Correlation Testing in Blood Bank
Mabel Adams reacted to Cliff for a topic
Here's the SOP I used, it may be a little dated.H-1-17_Method Comparison (JPTM).docx1 point -
At our facility, the Trainee has their own log in. The Trainer is responsible for assuring that all results are entered correctly. Should something be wrong, we would hold both responsible.1 point
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Immunoglobulin This question and answer was originally published on Lab Tests Guide. They have generously permitted us to repost here on our site. Please consider visiting their site: https://www.labtestsguide.com/ Submitter Cliff Category BloodBankTalk Submitted 10/03/20241 point
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DAT? I would do a panel, IS, RT incubation, 4C incubation......in tube. I say this because this is where the discrepancy is happening. I see you use Vision - have you done a regular panel on the instrument? Curious if it shows clear cut reactivity - or junkie, up the side-like reactivity? I would also do an ag type on the patient - even though they've been transfused......its' only 2 units, so, IF the pt is M neg, you should see MF if the units were M pos. ( we do this but don't report......it just give you an "idea" of what may or may not be going on......) If they type 3-4+ M pos with no MF, - you can - with a decent amount of certainty - eliminate M as a possibility. Remember...........M isn't the only trouble maker in the "cold". Could be one or both Lewis's, P1, I've actually seen a K react at RT - so, ya never know!1 point
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Case study book
Malcolm Needs reacted to Lorna Middleton for a topic
Sorry I'm just getting use to this site and how to reply! I am wanting to start off with easier ones and get more complicated. I'm trying to prepare for exams at a higher level which will include complicated case studies. I think both serological testing and clinical would be helpful? I am at Specialist level now but never worked in a reference lab and struggle with pan reactive panels and eluates/adsorption work and want to improve my theory so I can relate to complicated questions. 😊1 point -
Case study book
SbbPerson reacted to Lorna Middleton for a topic
Thank you so much I will have a look at that! 😊1 point -
Backtype discrepancy.. is it anti-a1?
John C. Staley reacted to Malcolm Needs for a topic
I CANNOT tell from the information you have given (not least because the phenotype of the reverse typing cells and the panel cells are unknown to me). I would very strongly suggest that you send samples to a Red Cell Reference Laboratory to get this sorted out, BEFORE the patient needs a transfusion in an emergency. From what you do tell us, I think the antibody/antibodies are unlikely to be fatally clinically significant, but it depends on the true specificity/specificities and the underlying pathology.1 point -
Hi Exlimey, this makes sense. Thank you for taking the time to explain it thoroughly. I appreciate it!1 point
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Case study book
Lorna Middleton reacted to SbbPerson for a topic
I have a book called "Antibody Identification: Art of science" . It's by the AABB, and it's chock full of case studies, over 500 pages of them, with questions for all of them.1 point -
Antibody Work-up
Ensis01 reacted to Malcolm Needs for a topic
I tend to think that there are a number of factors affecting the reaction, such as changes to the pH, rather than just dilution, that would change the equilibrium constant within the Law of Mass Action that governs antibody/antigen reactions, but pH is only one of them.1 point -
Case study book
Lorna Middleton reacted to AuntiS for a topic
For serological testing or for clinical situations?1 point -
Case study book
Lorna Middleton reacted to Malcolm Needs for a topic
Are you looking for really difficult cases, or more commonplace cases?1 point -
JCAHO - Issuing blood products
HMendel reacted to James Spears for a topic
We use un-validated lunch coolers just so that visitors/patients don't see someone walking through the halls with a bag of blood. OSHA reg is 1910.1030(g)(1)(i)(F) blood components issued for transfusion do not require a biohazard label.1 point -
Cliff: I just submitted my first question. Be easy on me1 point