Automated Red Cell Antibody Analysis. A Parallel Study

Perrault, P.; Högman, C.

doi:10.1159/000466654

Cited by 7 publications

(10 citation statements)

References 18 publications

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“…Experiments revealed that the LISPS system enhanced the reaction of MNS and Fya antibodies. Anti-K gave reactions equivalent to manual antiglobulin tests, but the system was slightly less sensitive than the BMC system in detecting weak anti-D, thus confirming the findings of Perrault and Hogman (1971).…”

supporting

confidence: 61%

“…Habibi et al (1973) and Perrault and Hogman (1971) overcame this problem by utilizing a selected panel of donors, but the provision of sufficient fully typed fresh cells for antibody screening is often difficult. Marsh et al (1968) and Moore (1969) found that glycerol frozen cells failed to form satisfactory rouleaux in the BMC system, although Kolberg and Nordhagen (1975) have reported satisfactory results with frozen cells in this system.…”

mentioning

confidence: 99%

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Improved antibody detection by the use of range expansion and longer filter wavelength in a low ionic strength-protamine sulphate Auto-Analyzer system.

Downie¹,

Voak²

1976

J Clin Pathol

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SYNOPSIS Range expansion, achieved by insertion of a variable resistance between the colorimeter and the recorder together with the use of 550 nm colorimeter filters, has resulted in markedly improved sensitivity for antibody detection, and improved sample identification, in a low ionic strength-protamine sulphate (LISPS) system. Range expansion also permits a lower concentration of red cells to be used, thus economizing on fully typed cells. Glycerol stored frozen cells were found to be only slightly less sensitive than fresh cells in this system.An automated antibody screening system should detect all antibodies of clinical significance with a sensitivity at least equal to and preferably better than the manual method it replaces. The bromelinmethyl cellulose (BMC) system described by Marsh et al (1968) has the disadvantage of not detecting weak antibodies to the enzyme degradable antigens MNS and Fya, and in our hands did not detect weak anti-K. Our attention was drawn to the low ionic strength-polybrene/protamine sulphate system described by Lalezari (1967;1968).In common with Dawes and Goldsmith (1975), we found that polybrene caused the aggregated cells to adhere to the glass coils, owing to the high degree of surface absorption of polybrene to glass, as noted by Greenwalt and Steane (1973). This resulted in cell baseline fluctuations, excessive 'carry-over', and poor sample identification. Reduction in the polybrene concentration to overcome these problems resulted in a loss of sensitivity. These difficulties were not experienced when protamine sulphate (Lalezari, 1967;Judd, 1971) was used, and this became the reagent of choice. Experiments revealed that the LISPS system enhanced the reaction of MNS and Fya antibodies. Anti-K gave reactions equivalent to manual antiglobulin tests, but the system was slightly less sensitive than the BMC system in detecting weak anti-D, thus confirming the findings of Perrault and Hogman (1971).

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supporting

confidence: 61%

mentioning

confidence: 99%

Improved antibody detection by the use of range expansion and longer filter wavelength in a low ionic strength-protamine sulphate Auto-Analyzer system.

Downie¹,

Voak²

1976

J Clin Pathol

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“…Marsh et al (1968) found that their BMC system reacted well with anti-S but anti-s was not tested. While Perrault and Hogman (1971) observed that the detection of anti-s on the AutoAnalyzer was less sensitive than the most appropriate manual technique. the anti-s described in this case was detected at a much higher titre on the AutoAnalyzer than by the indirect antiglobulin technique.…”

Section: Discussionmentioning

confidence: 98%

An example of anti-s causing mild haemolytic disease of the newborn

Davie¹,

Smith²,

White³

et al. 1972

J Clin Pathol

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“…Graduell differierende D u -Antigene können auch dem Erfahrenen bei der Abgrenzung Iow grade D u /d, insbesondere aber bei der Differenzierung high grade D U /D erhebliche Schwierigkeiten bereiten (4,5). -Die kontinuierliche Durchflußanalyse ermöglicht durch die photometrische Agglutinationsmessung den objektivierbaren Nachweis abgeschwächt reagierender Blutgruppenvarianten (6)(7)(8). Wir berichten über eine technische Erweiterung des Technicon-Geräts Autogrouper 16 C, die die kontinuierliche Erfassung des D-Allels D u und weiterer Rh-Varianten der Loci C und E ermöglicht sowie über Beobachtungen bei der Analyse von abgeschwächten Varianten Rh-Faktoren der 3 Rh-Loci.…”

Section: Introductionunclassified