Isaacman D J, Zhang Y, Reynolds E A, Ehrlich G D
Division of General Academic Pediatrics, Department of Pediatrics, University of Pittsburgh School of Medicine, Pittsburgh, PA, USA.
Pediatrics. 1998 May;101(5):813-6. doi: 10.1542/peds.101.5.813.
To evaluate the utility of a polymerase chain reaction (PCR)-based assay for identifying pneumococcal DNA in the blood of pediatric patients with suspected bacteremia.
Children evaluated at the Children's Hospital of Pittsburgh who were having blood drawn for culture had an additional 2 to 3 mL of blood (from the same sampling) obtained and placed in a sodium citrate tube for PCR processing (study group). The control group for this study consisted of children having blood drawn for biochemical analysis who were afebrile, well-appearing, and had no recent illnesses. Specimens were frozen at -70 degrees C and then batch-processed for PCR-based analyses with the JM201/202-204 primer/probe set. Amplified products were detected after liquid hybridization format wherein a 32P end-labeled probe was annealed to the amplified DNA and visualized by autoradiographic analysis after gel retardation.
Four hundred eighty study group patients and 103 controls had specimens tested by both PCR and blood culture. Twenty-six (5%) patients had a positive blood culture for a pathogenic organism (21 of which were Streptococcus pneumoniae). Twelve (57%) of the 21 patients with blood cultures positive for S pneumoniae also were positive by PCR. In addition, 206 study group patients and 16 controls with negative blood cultures had positive PCR results. A greater proportion of study group patients were PCR-positive/culture-negative than were controls (206/459 vs 16/103).
Although this assay currently lacks adequate sensitivity and specificity for clinical use, the high frequency of PCR-positive cases in patients with suspected bacteremia may indicate a greater role for S pneumoniae than had previously been appreciated. Further refinement of this assay as well as the development of a rapid PCR-based assay appears warranted.
评估基于聚合酶链反应(PCR)的检测方法在识别疑似菌血症儿科患者血液中肺炎球菌DNA的效用。
在匹兹堡儿童医院接受评估且正在抽血进行培养的儿童,从同一采样中额外采集2至3毫升血液,并置于柠檬酸钠管中用于PCR处理(研究组)。本研究的对照组由正在抽血进行生化分析、无发热、状态良好且近期无疾病的儿童组成。样本在-70℃下冷冻,然后使用JM201/202 - 204引物/探针组进行批量PCR分析。在液体杂交形式后检测扩增产物,其中将32P末端标记的探针与扩增的DNA退火,并在凝胶阻滞后通过放射自显影分析进行可视化。
480名研究组患者和103名对照的样本同时进行了PCR和血培养检测。26名(5%)患者的血培养中检测到致病微生物阳性(其中21例为肺炎链球菌)。21例血培养肺炎链球菌阳性的患者中有12例(57%)PCR检测也呈阳性。此外,206名研究组患者和16名血培养阴性的对照PCR结果呈阳性。研究组患者中PCR阳性/培养阴性的比例高于对照组(206/459对16/103)。
尽管该检测方法目前缺乏足够的敏感性和特异性用于临床应用,但疑似菌血症患者中PCR阳性病例的高频率可能表明肺炎链球菌的作用比之前认识到的更大。对该检测方法的进一步优化以及开发基于PCR的快速检测方法似乎是必要的。
