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通过降低感染婴儿利什曼原虫的犬体内S-腺苷甲硫氨酸合成酶(METK)基因的拷贝数,证明其对别嘌呤醇产生体内抗性。

Evidence for in vivo resistance against allopurinol in a dog infected with Leishmania infantum by reduction in copy numbers of the S-adenosylmethionine synthetase (METK) gene.

作者信息

Schäfer Ingo, Faucher Mathieu, Nachum-Biala Yaarit, Ferrer Lluís, Carrasco Marina, Kehl Alexandra, Müller Elisabeth, Naucke Torsten J, Baneth Gad

机构信息

LABOKLIN GmbH and Co. KG, Bad Kissingen, Germany.

Clinique Veterinaire Alliance, Bordeaux, France.

出版信息

Parasit Vectors. 2024 Dec 16;17(1):506. doi: 10.1186/s13071-024-06583-0.

Abstract

BACKGROUND

In Europe, canine leishmaniasis is commonly caused by Leishmania infantum. Allopurinol is the main drug for long-term management of the disease, and clinical relapses of L. infantum infection treated with this drug are described. Resistance to allopurinol has been demonstrated in-vitro, but there is only little knowledge on in vivo resistance in dogs.

FINDINGS

A two-year-old female spayed Akita Inu that was adopted from a breeding facility near Nice in France was initially diagnosed with primary immune-mediated hemolytic anemia. Immunosuppressive treatment was initiated, and the dog was referred for a second opinion to the Clinique Veterinaire Alliance in France. PCR testing for L. infantum was performed out of EDTA blood and IFA as well as ELISA testing out of serum. Resistance to allopurinol was associated with chromosome and gene copy number (CN) variations including a decrease in the S-adenosylmethionine synthetase (METK) gene CN.

RESULTS

The dog showed pale mucous membranes, fever (39.1 °C), and a relapse of the anemia. The diagnosis of leishmaniasis was based on the cytological finding of Leishmania amastigotes (bone marrow, spleen, liver), positive PCR testing, and positive IFAT serology. The dog was treated with allopurinol over a period of 1316 days and additionally received two cycles of Glucantime® (meglumine antimoniate), before samples were submitted to the LABOKLIN laboratory to test for resistance against allopurinol. The laboratory work-up revealed mild thrombocytopenia, mild hyperproteinemia with hyperglobulinemia, a marked elevation of the c-reactive protein, and decreased iron concentration. Serum protein electrophoresis showed a polyclonal peak in the gamma globulins. Serology was positive in both ELISA (21.5 LE) and IFAT (1:1024). Quantitative PCR testing of blood was positive with low numbers of Leishmania (10/ml blood) at the timepoint of suspicion for resistance. The urinary protein-to-creatinine ratio was markedly elevated (2.5) and xanthine crystalluria was detected. A CN level of below 3 is considered suspicious for resistance, as revealed in the described Akita Inu dog.

CONCLUSIONS

Relapse of L. infantum infection after applying allopurinol for 1316 days due to resistance was suspected clinically. Positive PCR testing, consistent hematological and biochemistry abnormalities, and reduction in the METK gene CN backed up the clinical suspicion of resistance. Dogs infected with allopurinol resistant strains of L. infantum may represent a great risk for infection of naïve dogs, cats, and humans.

摘要

背景

在欧洲,犬利什曼病通常由婴儿利什曼原虫引起。别嘌呤醇是该疾病长期治疗的主要药物,有关于用此药治疗婴儿利什曼原虫感染后临床复发的描述。体外已证实对别嘌呤醇存在耐药性,但对于犬体内耐药性的了解却很少。

研究结果

一只从法国尼斯附近的繁殖场收养的两岁已绝育秋田犬最初被诊断为原发性免疫介导性溶血性贫血。开始进行免疫抑制治疗,这只狗被转诊至法国的Clinique Veterinaire Alliance寻求第二种意见。用乙二胺四乙酸抗凝血进行婴儿利什曼原虫的PCR检测,并对血清进行间接荧光抗体试验(IFA)以及酶联免疫吸附测定(ELISA)检测。对别嘌呤醇的耐药性与染色体和基因拷贝数(CN)变异有关,包括S - 腺苷甲硫氨酸合成酶(METK)基因拷贝数减少。

结果

这只狗表现出黏膜苍白、发热(39.1℃)以及贫血复发。利什曼病的诊断基于利什曼原虫无鞭毛体的细胞学检查结果(骨髓、脾脏、肝脏)、PCR检测阳性以及间接荧光抗体试验血清学阳性。这只狗接受了1316天的别嘌呤醇治疗,另外还接受了两个周期的葡胺锑(Glucantime®)治疗,之后将样本提交给LABOKLIN实验室检测对别嘌呤醇的耐药性。实验室检查显示有轻度血小板减少、伴有高球蛋白血症的轻度高蛋白血症、C反应蛋白显著升高以及铁浓度降低。血清蛋白电泳显示γ球蛋白出现多克隆峰。ELISA(21.5 LE)和间接荧光抗体试验(1:1024)血清学均为阳性。在怀疑出现耐药性的时间点,血液定量PCR检测呈阳性,利什曼原虫数量较少(每毫升血液10个)。尿蛋白与肌酐比值显著升高(2.5),并检测到黄嘌呤结晶尿。在所描述的秋田犬中发现,CN水平低于3被认为有耐药性可疑。

结论

临床上怀疑在应用别嘌呤醇1316天后,由于耐药性导致婴儿利什曼原虫感染复发。PCR检测阳性、一致的血液学和生化异常以及METK基因拷贝数减少支持了对耐药性的临床怀疑。感染对别嘌呤醇耐药的婴儿利什曼原虫菌株的犬可能对未感染的犬、猫和人类构成重大感染风险。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a744/11650845/a2a4c7db6449/13071_2024_6583_Fig1_HTML.jpg

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