Mike,
"Of course outliers can be identified using duplicates. If the duplicates do not agree closely you repeat the test."
Maybe I am a bear of little brain.
How do you identify the outlier at the time of initial duplication? If you do, would you not be able to report the non-outlier thus negating the requirement for a repeat?
-----Original Message-----
From: Clinical biochemistry discussion list
[mailto:[log in to unmask]]On Behalf Of COLLINS MICHAEL
(RM1) Norfolk and Norwich University Hospital
Sent: 24 March 2010 09:49
To: [log in to unmask]
Subject: Re: Manually improving precision?
Of course outliers can be identified using duplicates. If the duplicates do not agree closely you repeat the test.
Mike Collins
BMS3
Biochemistry Automation
Norfolk & Norwich University Hospital
England
[log in to unmask]
http://www.nnuh.nhs.uk/
-----Original Message-----
From: Clinical biochemistry discussion list [mailto:[log in to unmask]] On Behalf Of Roger Ekins
Sent: 23 March 2010 21:14
To: [log in to unmask]
Subject: Re: Manually improving precision?
Gordon. Andy, Johnathan, et al,
Duplicates certainly reduce the s.d. by a factor of sqrt 2, thereby
increasing intra-assay precision. Duplicates also enabled us to
identify a 'missed' tube, i.e. one in which a key reagent had been
omitted. (This was obviously in the days when everything was done by
hand, before automatic analysers became available.) But outliers
could not generally be identified using duplicates, because it might
not be evident which of the duplicates was the outlier. Also -
using duplicates - we could routinely calculate the intra-assay
precision/imprecision profile, which provided a form of internal
quality control.
But how, Gordon, used you to determine inter-assay imprecision? This
contains statistical errors resulting from intra-assay imprecision.
Of course one could calculate the inter-assay component, knowing the
intra-assay component, and I recall doing this. But whether one uses
singletons or duplicates in an assay will alter the overall
inter-assay precision.
On a different (semantic) point, I understand why purists prefer to
use the term 'imprecision' rather than ,'precision' in this context.
This seems to be because we generally represent precision/imprecision
by the s.d or c.v. of replicate measurements.
But the use of the term precision in this context has a long history;
statisticians concerned with bioassays would refer to the "index of
precision" rather than the "index of imprecision".
And I also wonder whether purists would refer to the "insensitivity"
of an assay because the detection limit is indicated the
'imprecision' with which we measure an analyte concentration of zero?
Roger
>Dear Andy and Jonathan
>Within-assay replication decreases the within-run component of
>variation by a factor related to the square root of the number of
>replicates. It does not affect the between-run and
>between-laboratory components of variation.
>It was widely used in bioassays and radioimmunoassay, but the
>primary use was to detect blunders and fliers; not to reduce
>imprecision.
>Best wishes
>Gordon Challand
>----- Original Message ----- From: "Jonathan Kay"
><[log in to unmask]>
>To: <[log in to unmask]>
>Sent: Tuesday, March 23, 2010 11:12 AM
>Subject: Re: Manually improving precision?
>
>
>Analysis in duplicate was common in immunoassay and some other
>methods until very recently. My feeling is that it was done more to
>catch blunders and flyers than to improve precision.
>
>Where are people currently using duplicate in clinical assays?
>
>Jonathan
>
>On 22 Mar 2010, at 15:47, Andy Minett wrote:
>
>>Dear All,
>>
>>I have recently been reading about the tightening of quality requirements in
>>proficiency testing for glycated haemoglobin in America
>>(http://james.westgard.com/the_westgard_rules/2010/02/gutcheck-
>>hba1c.html ). One of the issues raised here is that many platforms do not
>>deliver the necessary imprecision to meet current quality requirements, let
>>alone future improvements.
>>
>>In fear of making a rather banal suggestion, has anyone looked at "manually"
>>(elaboration below) reducing the imprecision of an analyser? In fact, I am so
>>sure this approach has been considered and rejected, the question I am really
>>asking is: what are the drawbacks of this approach, and can the mailbase
>>provide me with references that discuss it (my own searches have been
>>unfruitful).
>>
>>By "manually reducing imprecision" what I mean is taking multiple
>>simultaneous
>>readings and reporting the average of those as the test result. In
>>an unrelated
>>(i.e. not Biochemistry related) mathematical project, I needed to
>>find a way of
>>minimising the scatter of data from a Normal Random number generator with
>>fixed Mean and CV. Through mass data testing I calculated the reduction in
>>scatter (CV) to be closely estimated by:
>>
>>% reduction in CV = (1-1/(n^0.5)) * 100
>>
>>(where n = number of replicate measurements averaged)
>>
>>Using this in my project, I was able to reduce the CV of the number generator
>>by 80% by averaging 25 results from it.
>>
>>Imagining a hypothetical glycated haemoglobin analyser that has a stable CV
>>of 3% say, taking the average of 4 simultaneous analyses of each sample
>>would reduce the CV of the method by 50%; to 1.5%.
>>
>>What are the drawbacks to using this approach in blood analysis? Other than
>>the approach being n times as costly as single-result analysis.
>>
>>Best regards,
>>Andy Minett
>>
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>community working in clinical biochemistry.
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>internet. Views expressed are those of the individual and they are
>responsible for all message content.
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--
Prof Roger Ekins, PhD DSc FRS
Windeyer Institute of Medical Science
University College London
London W1T 4JF
Phone +44 20 7679 9410
Fax +44 20 7679 9407
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