1.Confirmation of pipetting performances for fully-open automatic biochemistry analyzers.
Chinese Journal of Medical Instrumentation 2005;29(4):277-282
This paper introduces a kind of evaluation method in pipetting performance on new fully automated biochemistry analyzers by experiments. The performance of sample pipetting volume is confirmed by dye dilution method, the performance of reagent pipetting volume and dummy volume is done by weighing method. Meanwhile, researches and comparative researches on dummy volumes in different conditions have been made, providing valuable reference for clinical applications of automatic biochemistry analyzers.
Automation, Laboratory
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instrumentation
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methods
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Biochemistry
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instrumentation
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methods
2.Modeling and implementation method for the automatic biochemistry analyzer control system.
Dong WANG ; Wan-cheng GE ; Chun-lin SONG ; Yun-guang WANG
Chinese Journal of Medical Instrumentation 2009;33(3):217-220
In this paper the system structure The automatic biochemistry analyzer is a necessary instrument for clinical diagnostics. First of is analyzed. The system problems description and the fundamental principles for dispatch are brought forward. Then this text puts emphasis on the modeling for the automatic biochemistry analyzer control system. The objects model and the communications model are put forward. Finally, the implementation method is designed. It indicates that the system based on the model has good performance.
Autoanalysis
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instrumentation
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methods
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Biochemistry
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instrumentation
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methods
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Equipment Design
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Models, Theoretical
3.Development of a fully-automated biochemical analysis system intended for primay medical units.
Chuanfen XIE ; Zhihong WANG ; Wei WANG
Chinese Journal of Medical Instrumentation 2011;35(5):348-351
A fully-automated biochemical analysis system is developed, intending for primary medical units. It features high reliability, high usability, strong adaptability, low operation cost, low maintenance cost, and low requirements for operators.
Automation
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instrumentation
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methods
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Biochemistry
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instrumentation
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methods
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Equipment Design
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Equipment and Supplies, Hospital
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Hospitals, Rural
4.Performance Evaluation of the LABGEO PT10 Point-of-care Chemistry Analyzer.
Tae Dong JEONG ; Woochang LEE ; Sail CHUN ; Won Ki MIN
Journal of Laboratory Medicine and Quality Assurance 2013;35(2):70-80
BACKGROUND: The Samsung LABGEO PT10 (Samsung Electronics, Korea) has been developed as a point-of-care testing (POCT) chemistry analyzer. We evaluated the performance of the Samsung LABGEO PT Biochemistry Test 15 (Samsung Electronics) and the HbA1c Test (Samsung Electronics), which are dedicated cartridges for the LABGEO PT10. METHODS: Based on the Clinical and Laboratory Standards Institute guidelines, the precision, linearity, and methodology were evaluated for seven chemistry analytes (cholesterol, triglycerides, HDL cholesterol, blood urea nitrogen, creatinine, amylase, and hemoglobin A1c). All the analytes, except for hemoglobin A1c, were obtained from three different types of samples: whole blood, plasma, and serum, to evaluate matrix effects. RESULTS: In the precision analysis, both within-run and total-run coefficients of variation were less than 10% for the seven analytes. Dose curves for the seven analytes were linear in the clinically relevant concentration ranges. The methodology study yielded correlation coefficients > or =0.98 for the seven comparisons of the LABGEO PT10 cartridge tests with other methods. Except for HDL cholesterol, the percentage differences between test results obtained from whole blood, plasma, and serum, were within +/-10%. The concentrations of HDL cholesterol measured in whole blood samples were 0.9 mg/dL and 5.6 mg/dL higher than those measured in plasma and serum specimens, respectively. CONCLUSIONS: The LABGEO PT10 showed suitable analytical performance with respect to precision and linearity and demonstrated a good correlation with automated chemistry analyzer. With the additional benefits of a short turnaround time and ease of use, the LABGEO PT10 is an acceptable POCT chemistry analyzer.
Amylases
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Biochemistry
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Blood Urea Nitrogen
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Chemistry*
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Cholesterol, HDL
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Creatinine
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Methods
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Plasma
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Point-of-Care Systems
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Triglycerides
5.Determination of alpha-glucosidase activity in seminal plasma by semi-automatic biochemistry analyzer.
Jin-chun LU ; Hui-ru XU ; Yu-feng HUANG
National Journal of Andrology 2007;13(9):791-794
OBJECTIVETo establish a method of determining alpha-glucosidase activity in seminal plasma by semi-automatic biochemistry analyzer.
METHODSAlpha-glucosidase activity in seminal plasma from 51 men with normal semen parameters in routine semen analysis were detected by semi-automatic biochemistry analyzer and manual glucose oxidase method, respectively. Then, the intra-assay and inter-assay coefficient variation (CV) and normal reference value were calculated. In the meanwhile, the correlation between the two methods was analyzed.
RESULTSThe intra-assay CVs of 2 seminal plasma samples with different alpha-glucosidase activity detected by semi-automatic biochemistry analyzer were 12.63% and 9.13%, and the inter-assay CVs were 10.67% and 13.49%, respectively. The normal reference value for seminal alpha-glucosidase activity detected with semi-automatic biochemistry analyzer ranged from 102.28 to 555.08 U/L. There was a significantly positive correlation between the semi-automatic biochemistry analyzer and the manual glucose oxidase method (r = 0.792, P < 0.01).
CONCLUSIONThe method of determining alpha-glucosidase activity in seminal plasma by semi-automatic biochemistry analyzer, with its simplicity, less cost of time and reagents, and more reliable result, could be applied to clinical laboratory medicine.
Adult ; Biochemistry ; instrumentation ; methods ; Humans ; Male ; Reference Values ; Reproducibility of Results ; Semen ; enzymology ; alpha-Glucosidases ; analysis ; metabolism
6.Pharmacokinetics of tilmicosin in healthy pigs and in pigs experimentally infected with Haemophilus parasuis.
Ling ZHANG ; Li ZHAO ; Yonghong LIU ; Junfeng LIU ; Xianqiang LI
Journal of Veterinary Science 2017;18(4):431-437
A comparative in vivo pharmacokinetic (PK) study of tilmicosin (TIL) was conducted in 6 crossbred healthy pigs and 6 crossbred pigs infected with Haemophilus (H.) parasuis following oral administration of a single 40 mg/kg dose. The infected model was established by intranasal inoculation and confirmed by clinical signs, blood biochemistry, and microscopic examinations. Plasma TIL concentrations were determined by a validated high-performance liquid chromatography method with ultraviolet detection at 285 nm. PK parameters were calculated by using WinNonlin software. After TIL administration, the main PK parameters of TIL in healthy and H. parasuis-infected pigs were as follows: Area under the concentration-time curve, maximal drug concentration, half-life of the absorption phase, half-life of the distribution phase, and half-life of the elimination phase were 34.86 ± 9.69 vs. 28.73 ± 6.18 µg · h/mL, 1.77 ± 0.33 vs. 1.67 ± 0.28 µg/mL, 2.27 ± 0.45 vs. 2.24 ± 0.44 h, 5.35 ± 1.40 vs. 4.61 ± 0.35 h, and 43.53 ± 8.17 vs. 42.05 ± 9.36 h, respectively. These results of this exploratory study suggest that there were no significant differences between the PK profiles of TIL in the healthy and H. parasuis-infected pigs.
Absorption
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Administration, Oral
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Biochemistry
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Chromatography, Liquid
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Haemophilus parasuis*
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Haemophilus*
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Half-Life
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Methods
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Pharmacokinetics*
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Plasma
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Swine*
7.In vitro and in vivo Efficacy of New Blue Light Emitting Diode Phototherapy Compared to Conventional Halogen Quartz Phototherapy for Neonatal Jaundice.
Yun Sil CHANG ; Jong Hee HWANG ; Hyuk Nam KWON ; Chang Won CHOI ; Sun Young KO ; Won Soon PARK ; Son Moon SHIN ; Munhyang LEE
Journal of Korean Medical Science 2005;20(1):61-64
High intensity light emitting diodes (LEDs) are being studied as possible light sources for the phototherapy of neonatal jaundice, as they can emit high intensity light of narrow wavelength band in the blue region of the visible light spectrum corresponding to the spectrum of maximal bilirubin absorption. We developed a prototype blue gallium nitride LED phototherapy unit with high intensity, and compared its efficacy to commercially used halogen quartz phototherapy device by measuring both in vitro and in vivo bilirubin photodegradation. The prototype device with two focused arrays, each with 500 blue LEDs, generated greater irradiance than the conventional device tested. The LED device showed a significantly higher efficacy of bilirubin photodegradation than the conventional phototherapy in both in vitro experiment using microhematocrit tubes (44 +/-7% vs. 35 +/-2%) and in vivo experiment using Gunn rats (30 +/-9% vs. 16 +/-8%). We conclude that high intensity blue LED device was much more effective than conventional phototherapy of both in vitro and in vivo bilirubin photodegradation. Further studies will be necessary to prove its clinical efficacy.
Animals
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Bilirubin/*metabolism
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Biochemistry/*methods
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Gallium/pharmacology
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Hematocrit
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In Vitro
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*Light
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Phototherapy/*methods
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Rats
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Rats, Gunn
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Research Support, Non-U.S. Gov't
8.Application Fourier transform near infrared spectrometer in rapid estimation of soluble solids content of intact citrus fruits.
Hui-shan LU ; Hui-rong XU ; Yi-bin YING ; Xia-ping FU ; Hai-yan YU ; Hai-qing TIAN
Journal of Zhejiang University. Science. B 2006;7(10):794-799
Nondestructive method of measuring soluble solids content (SSC) of citrus fruits was developed using Fourier transform near infrared reflectance (FT-NIR) measurements collected through optics fiber. The models describing the relationship between SSC and the NIR spectra of citrus fruits were developed and evaluated. Different spectra correction algorithms (standard normal variate (SNV), multiplicative signal correction (MSC)) were used in this study. The relationship between laboratory SSC and FT-NIR spectra of citrus fruits was analyzed via principle component regression (PCR) and partial least squares (PLS) regression method. Models based on the different spectral ranges were compared in this research. The first derivative and second derivative were applied to all spectra to reduce the effects of sample size, light scattering, instrument noise, etc. Different baseline correction methods were applied to improve the spectral data quality. Among them the second derivative method after baseline correction produced best noise removing capability and yielded optimal calibration models. A total of 170 NIR spectra were acquired; 135 NIR spectra were used to develop the calibration model; the remaining spectra were used to validate the model. The developed PLS model describing the relationship between SSC and NIR reflectance spectra could predict SSC of 35 samples with correlation coefficient of 0.995 and RMSEP of 0.79 degrees Brix.
Biochemistry
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methods
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Calibration
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Citrus
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metabolism
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Least-Squares Analysis
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Light
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Models, Statistical
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Regression Analysis
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Reproducibility of Results
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Scattering, Radiation
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Spectroscopy, Fourier Transform Infrared
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methods
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Spectroscopy, Near-Infrared
9.Synthesis and paste properties of octenyl succinic anhydride modified early Indica rice starch.
Xiao-yan SONG ; Qi-he CHEN ; Hui RUAN ; Guo-qing HE ; Qiong XU
Journal of Zhejiang University. Science. B 2006;7(10):800-805
Octenyl succinic anhydride (OSA) modified early Indica rice starch was prepared in aqueous slurry systems using response surface methodology. The paste properties of the OSA starch were also investigated. Results indicated that the suitable parameters for the preparation of OSA starch from early Indica rice starch were as follows: reaction period 4 h, reaction temperature 33.4 degrees C, pH of reaction system 8.4, concentration of starch slurry 36.8% (in proportion to water, w/w), amount of OSA 3% (in proportion to starch, w/w). The degree of substitution was 0.0188 and the reaction efficiency was 81.0%. The results of paste properties showed that with increased OSA modification, the starch derivatives had higher paste clarity, decreased retrogradation and better freeze-thaw stability.
Biochemistry
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methods
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Chemical Phenomena
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Chemistry, Physical
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Freezing
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Hydrogen-Ion Concentration
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Light
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Models, Statistical
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Oryza
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metabolism
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Starch
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chemistry
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Succinic Anhydrides
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analysis
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chemistry
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Temperature
10.Establishment of a protein misfolding cyclic amplification for PrPSc.
Jun HAN ; Lu HAN ; Qi SHI ; Song SHI ; Xin WANG ; Bao-Yun ZHANG ; Xiao-Ping DONG
Chinese Journal of Experimental and Clinical Virology 2007;21(3):202-204
OBJECTIVETo establish a methodology of protein misfolding cyclic amplification (PMCA) and utilize in the detection of PrP(Sc) in brain tissues from prion diseases.
METHODSDifferent amounts of Scrapie 263K agent bulk were mixed with brain homogenates of health hamsters and treated with repeated incubation/sonication for 10 to 15 cycles. The proteinase K-resistant PrP(Sc) was evaluated with Western Blot.
RESULTSIn this experimental situation, 263K agent replicated rapidly in vitro, utilizing hamsters' brains as the medium. With the established PrP(Sc)-PMCA technique, PrP(Sc) signals in the preparations containing less than 10(-5) diluted 263K bulk could be detected. Compared with conveniently used immuno-blot assay, the sensitivity of PrP(Sc)-PMCA for PrP(Sc) was 10(5) to 10(6)-fold increased. It has been also shown that homogenates of cerebellar and brain stem could be used as the medium for PrP(Sc) replication.
CONCLUSIONA rapidly replicating method for PrP(Sc), PrP(Sc)-PMCA, was successfully established, providing a new approach for early diagnosis of prion diseases and research on the biological features of prion.
Animals ; Biochemistry ; methods ; Blotting, Western ; Brain ; metabolism ; pathology ; Cricetinae ; PrPSc Proteins ; analysis ; chemistry ; Prion Diseases ; diagnosis ; metabolism ; Protein Folding ; Reproducibility of Results ; Sensitivity and Specificity