RESUMO
BACKGROUND AND PURPOSE: The standard dosimetry system of medical accelerators in radiotherapy consists of an ionization chamber, an electrometer, and cables. Guidance for TG-51 reference dosimetry reported that the electrometer correction factor (Pelec ) should be checked every few years. Therefore, continuous Pelec measurements have not been reported. The purpose of this study is to measure the Pelec with a charge generator at our institution and to evaluate variations over time. The measurements are compared with calibration data given by an Accredited Dosimetry Calibration Laboratory (ADCL). MATERIALS AND METHODS: We used four reference-class electrometers: RT521R (RTQM system/EMF Japan), Model 35040 (FLUKE), RAMTEC Duo (Toyo medic), and UNIDOS-E (PTW). Each electrometer was connected to the charge generator, and the required charge was applied. The measurement points used were the same as those used for calibration by the ADCL. From the measured charges at each point, the Pelec was obtained from the slope of the linear regression function. The measurements were repeated over a 3-month period to evaluate variations over time for each electrometer. Additionally, error budgets for the Pelec measurements were estimated, and the overall uncertainty was determined. RESULTS: The measured Pelec values were 1.0000, 0.9995, 1.0009/0.9999, and 0.9995/0.9998 for RT521R, Model 35040, the low/medium (L/M) ranges of RAMTEC Duo, and the L/M ranges of UNIDOS-E, respectively. The measured Pelec values agreed within 0.1% with those given by the ADCL. We found a small drift in the measurements for one electrometer. Additionally, the uncertainty considered was 0.26% for k = 2 (k, coverage factor). CONCLUSION: In this study, stable Pelec values were obtained for four electrometers using a charge generator over a three-month period. The measured Pelec values were within the overall uncertainty stated in the electrometer guidelines. However, performing periodic measurements for the Pelec was able to help in detecting small errors.
Assuntos
Radiometria , Humanos , Radiometria/métodos , Calibragem , JapãoRESUMO
IncX3 and IncL plasmids have been named as catalysts advancing dissemination of blaOXA-181 and blaOXA-48 genes. However, their impact on the performance of host cells is vastly understudied. Genetic characteristics of blaOXA-48- and blaOXA-181-containing Klebsiella pneumoniae (EFN299), Klebsiella quasipneumoniae (EFN262), and Enterobacter cloacae (EFN743) isolated from clinical samples in a Ghanaian hospital were investigated by whole-genome sequencing. Transfer of plasmids by conjugation and electroporation, plasmid stability, fitness cost, and genetic context of blaOXA-48, blaOXA-181, and blaDHA-1 were assessed. blaOXA-181 was carried on two IncX3 plasmids, an intact 51.5-kb IncX3 plasmid (p262-OXA-181) and a 45.3-kb IncX3 plasmid (p743-OXA-181) without replication protein sequence. The fluoroquinolone-resistant gene qnrS1 region was also excised, and unlike in p262-OXA-181, the blaOXA-181 drug-resistant region was not found on a composite transposon. blaOXA-48 was carried on a 74.6-kb conjugative IncL plasmid with unknown ~10.9-kb sequence insertion. This IncL plasmid proved to be highly transferable, with a conjugation efficiency of 1.8 × 10-2. blaDHA-1 was present on an untypeable 22.2 kb genetic structure. Plasmid stability test revealed plasmid loss rate between 4.3% and 12.4%. The results also demonstrated that carriage of IncX3-blaOXA-181 or IncL-blaOXA-48 plasmids was not associated with any fitness defect, but rather an enhanced competitive ability of host cells. This study underscores the significant contribution of IncX3 and IncL plasmids in the dissemination of resistance genes and their efficient transfer calls for regular monitoring to control the expansion of resistant strains. IMPORTANCE The growing rate of antibiotic resistance is an important global health threat. This threat is exacerbated by the lack of safe and potent alternatives to carbapenems in addition to the slow developmental process of newer and effective antibiotics. Infections by carbapenem-resistant Gram-negative bacteria are becoming almost untreatable, leading to poor clinical outcomes and high mortality rates. OXA-48-like carbapenemases are one of the most widespread carbapenemases accounting for resistance among Enterobacteriaecae. We characterized OXA-48- and OXA-181-producing Enterobacteriaecae to gain insights into the genetic basis and mechanism of resistance to carbapenems. Findings from the study showed that the genes encoding these enzymes were carried on highly transmissible plasmids, one of which had sequences absent in other similar plasmids. This implies that mobile genetic elements are important players in the dissemination of resistance genes. Further characterization of this plasmid is warranted to determine the role of this sequence in the spread of resistance genes.