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Featured researches published by Sm Cue.


Veterinary Microbiology | 2009

Description of outcomes of experimental infection with feline haemoplasmas: Copy numbers, haematology, Coombs' testing and blood glucose concentrations

Séverine Tasker; Iain R. Peters; Kostas Papasouliotis; Sm Cue; Barbara Willi; Regina Hofmann-Lehmann; Tj Gruffydd-Jones; Toby G Knowles; Michael J. Day; Christopher R Helps

The aim of this study was to compare blood copy, haematological and glucose values between cats experimentally infected with either Mycoplasma haemofelis (Group HF: 10 cats), ‘Candidatus M. haemominutum’ (Group HM: 3 cats) or ‘Candidatus M. turicensis’ (Group TU: 3 cats). Blood samples were collected regularly up to 85 days post-infection (DPI) for haemoplasma real-time quantitative PCR, haematology, Coombs’ testing and blood glucose measurement. Statistical analysis was performed using a general linear model (ANOVA) appropriate for a repeated measures experiment with significance set as P < 0.05. Cats in Group TU had significantly lower blood copy numbers than cats in Group HF (P < 0.001) and HM (P < 0.001). All Group HF cats developed anaemia (often severe), macrocytosis and evidence of erythrocyte-bound antibodies whereas Groups HM and TU cats did not. Group HF had significantly lower PCVs, haemoglobin concentrations and red blood cell counts, and significantly higher mean cell volumes, than Groups HM and TU. In Group HF, erythrocyte-bound antibodies reactive at 4 °C (both IgM and IgG) appeared between 8 and 22 DPI and persisted for two to four weeks, whereas those reactive at 37 °C (primarily IgG) appeared between 22 and 29 DPI and persisted for one to five weeks. In most cats antibodies appeared after the fall in haemoglobin started. Although Group TU had significantly lower glucose concentrations than Groups HF (P = 0.006) and HM (P = 0.027), mean blood glucose concentrations remained within the reference range in all groups. This study demonstrates that M. haemofelis infection, in contrast to ‘Candidatus M. haemominutum’ and ‘Candidatus M. turicensis’ infection, can result in a severe macrocytic anaemia and the development of cold and warm reactive erythrocyte-bound antibodies.


Journal of Small Animal Practice | 2012

Measurement of prothrombin time and activated partial thromboplastin time in citrated whole blood samples from clinically ill dogs following storage

Christina L Maunder; Marta T Costa; Sm Cue; Em Crawford; Kostas Papasouliotis; Kate Murphy

OBJECTIVES To assess the reliability of prothrombin time and activated partial thromboplastin time results generated from citrated whole blood samples following short-term storage at room temperature. METHODS Clotting times were measured in blood samples from 40 dogs that showed a variety of clinical signs. Before measurement of prothrombin time and activated partial thromboplastin time in citrated plasma, whole blood samples were split in three aliquots; one was processed within 30 minutes of collection (fresh) while the remaining two were stored unseparated at room temperature for 24 (24RT) or 48 (48RT) hours. RESULTS The median prothrombin time for the 24RT (7 seconds) and 48RT (7·2 seconds) samples were not significantly different to those obtained from the fresh (7·1 seconds) samples but the median activated partial thromboplastin time for the 24RT (12·6 seconds) and 48RT (12 seconds) samples were significantly shorter than those obtained from the fresh samples (14·2 seconds). CLINICAL SIGNIFICANCE Storage of citrated whole blood at room temperature for 24 or 48 hours did not significantly alter the measurement of prothrombin time but resulted in significantly shorter activated partial thromboplastin time results. Extrapolating from these findings, it is proposed that unseparated clinical samples that are submitted to an external diagnostic laboratory for the performance of clotting times, may generate reliable prothrombin time but unreliable activated partial thromboplastin time results.


Veterinary Clinical Pathology | 2006

Comparison of white blood cell differential percentages determined by the in‐house LaserCyte hematology analyzer and a manual method

Kostas Papasouliotis; Sm Cue; Em Crawford; Mark D.G. Pinches; Michel Dumont; Ken Burley


Research in Veterinary Science | 2008

Measurement of prothrombin time (PT) and activated partial thromboplastin time (APTT) on canine citrated plasma samples following different storage conditions

Francesca Rizzo; Kostas Papasouliotis; Em Crawford; Sj Dodkin; Sm Cue


Journal of Small Animal Practice | 2003

Analysis of canine and feline haemograms using the VetScan HMT analyser

E Dewhurst; Em Crawford; Sm Cue; Sj Dodkin; Ac German; Kostas Papasouliotis


Veterinary Clinical Pathology | 1999

Analysis of Feline, Canine and Equine Hemograms Using the QBC VetAutoread

Kostas Papasouliotis; Sm Cue; Mary Graham; A H Sparkes; Tj Gruffydd-Jones


Journal of Small Animal Practice | 2008

A retrospective study of canine D-dimer concentrations measured using an immunometric "Point-of-Care" test.

E Dewhurst; Sm Cue; Em Crawford; Kostas Papasouliotis


Research in Veterinary Science | 2008

Effect of storage on microcytosis observed in dogs with portosystemic vascular anomalies

Mark R. Goodfellow; Kostas Papasouliotis; Sm Cue; Em Crawford; Edward J Hall


Archive | 2012

Evaluation of EDTA haematology tubes for the measurement of D-dimer concentration in dogs

Marta T Costa; Sm Cue; Em Crawford; Stephen J Dodkin; Kostas Papasouliotis


Archive | 2012

Measurement of D-dimer concentrations in citrated whole blood samples following storage at room temperature.

Marta T Costa; Sm Cue; Em Crawford; Stephen J Dodkin; Kostas Papasouliotis

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Sj Dodkin

University of Bristol

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