• 대한화학회지
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• 제46권6호
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• pp.535-540
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• 2002

남조류 독소인 마이크로시틴은 호수에서 매우 미량 존재하기 때문에 이를 정확히 정량 분석하기가 쉽지 않다. 본 연구에서는 소양호에서 채취한 물시료 중에 포함된 남조류 독소, 마이크로시틴을 정량 분석하기 위하여 두 가지 서로 다른 정량 분석법을 시도하였으며 이 둘의 정량 결과를 비교${\cdot}$분석 하였다. 첫째는 고체상 추출과 HPLC(High Performance Liquid Chromatography)를 이용한 분석법을 이용하였으며 둘째는 마이크로시틴의 단일클론항체를 이용한 효소면역흡착분석법(Enzyme-Linked Immunosorbent Assay,ELISA)을 이용하였다.

• Journal of Microbiology and Biotechnology
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• 제16권2호
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• pp.205-211
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• 2006

A quantitative analytical method to detect new lines of genetically modified (GM) maize, NK603 and TC1507, has been developed by using a real-time polymerase chain reaction (PCR). To detect these GM lines, two specific primer pairs and probes were designed. A plasmid as a reference molecule was constructed from an endogenous DNA sequence of maize, a universal sequence of a cauliflower mosaic virus (CaMV) 35S promoter used in most GMOs, and each DNA sequence specific to the NK603 and TC1507 lines. For the validation of this method, the test samples of 0, 0.1, 0.5, 1.0, 3.0, 5.0, and 10.0% each of the NK603 and TC1507 GM maize were quantitated. At the 3.0% level, the biases (mean vs. true value) for the NK603 and TC1507 lines were 3.3% and 15.7%, respectively, and their relative standard deviations were 7.2% and 5.5%, respectively. These results indicate that the PCR method developed in this study can be used to quantitatively detect the NK603 and TC1507 lines of GM maize.

• 웰빙융합연구
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• 제5권1호
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• pp.37-46
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• 2022

Purpose: This study examines the history of the evolution of MS analysis and intends to consider the future direction of technological development through the difference from the latest technology, SIFT-MS. Research design, data and methodology: A method of analysis will be described in detail at the below by SIFT-MS (Selected Ion Flow Mass Spectrometry), which is a technology developed by a company called SIFT Technologies. Results: The initial concept of mass spectrometry was begun in the late 1890s, and it continues to evolve even after the 21st century through the ripening stage of the 20th century. The development process of mass spectrometry by year has been described in detail in the Main text. Conclusions: Mass spectrometry, qualitative and quantitative analysis of substances plays a very important role in the research and medical fields. The development of these analytical methods is expected to continue in the future, and faster and more accurate qualitative analysis and mass spectrometry will be developed than the level currently reached. In addition, it is expected that hardware and software will be configured so that non-analysis experts can handle it easily, and it will be used as a technology that is more closely related to our lives.

• 한국환경농학회지
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• 제34권1호
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• pp.52-56
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• 2015

BACKGROUND: Three commercial biopesticides containing derris extract, which is permitted as a commercial biopesticide substances by the Environmentally-friendly Agriculture Promotion Act, have been marketed in Korea. But, the quantitative analytical method of active substances for crop protection in biopesticides containing derris extract has not known. METHODS AND RESULTS: Solid phase extraction (SPE) cartridge clean-up method for the quantitative analysis of rotenone and deguelin in biopesticides containing derris extract was developed and validated by ultra-performance liquid chromatography (UPLC). The clean-up method was established using hydrophilic lipophilic balance (HLB) SPE cartridges for the bioactive substances in biopesticides containing derris extract, and the eluate was analyzed to quantify the rotenone and deguelin by the UPLC. LOQ and recovery rates of rotenone and deguelin were 0.085 and 0.044 mg/L, 95.7 and 93.3%, respectively. The content of rotenone and deguelin in three biopesticides containing derris extract were analyzed by the developed method, the results showed 0.001-0.236 and

• 농약과학회지
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• 제13권4호
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• pp.223-231
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• 2009

본 연구는 살균제 fenhexamid의 잔류분석을 대부분의 농작물에 적용할 수 있도록 대표 작물을 이용한 fenhexamid의 단성분 정밀 분석법을 개발하고자 하였다. 대표 작물로는 배추, 감귤, 사과, 고추로 선정하였고, 마쇄한 농작물 시료에 acetone을 가한 후 진탕하여 잔류물을 추출하였다. 추출액을 감압농축 한 뒤, 농축물을 포화식염수와 증류수로 희석하고 dichloromethane으로 분배하였다. 분배액을 농축하고 ethyl acetate/0.1 % acetic acid 함유 hexane 혼합액[15:85, (v/v)]으로 용리하는 Florisil 크로마토그래피법으로 정제한 후 농축한 다음 HPLC로 분석하는 방법을 확립하였다. Fenhexamid의 정량한계(LOQ ; Limit of Quantitation)는 1 ng(S/N>10)이었고, 분석정량한계(MQL ; Method Quantitative Limit)는 0.01 mg/kg이었다. 무처리 시료에 fenhexamid 표준용액을 2수준(10MQL과 50MQL) 3반복으로 처리하여, 확립된 전체 분석과정을 거친 후, 회수율을 산출한 결과는 85.2~94.8%이었으며, 농산물 시료에 관계없이 반복 간 분석오차는 10% 미만이었다.

• 분석과학
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• 제30권5호
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• pp.252-261
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• 2017

천연방사성핵종을 함유한 물질들은 인간 활동에 의해 인위적인 조작과정을 거치면서 농축되는 경우 방사선 노출에 따른 위해를 증가시킬 수 있다. 본 연구는 다양한 전처리 방법 및 분석 방법 간 비교를 통해 분석정확도를 평가하고 실내 건축자재 중 $^{232}Th$, $^{235}U$, $^{238}U$의 천연방사성핵종을 분석하기 위한 최적의 분석 방법을 확립하고자 하였다. ICP-MS를 이용한 실내 건축자재 중 천연방사성핵종 분석방법을 확립하기 위하여, 인증표준물질 5종을 왕수, 불산, 과염소산의 습식산화법과 용융법의 전처리법에 따른 U, Th의 분석 정확도 및 정밀도를 평가하였고, 최적의 전처리법으로써 용융법과 $Fe(OH)_3$ 공침법을 선정하였다. 확립된 분석방법을 석고보드, 벽돌, 시멘트, 페인트, 타일과 벽지 총 51 종의 실내 건축자재 시료에 적용하여 천연방사성핵종의 농도를 정량 분석하였다. 또한 동일한 시료에 대해 감마분광분석법 중 간접측정법을 사용하여 $^{238}U$, $^{232}Th$의 농도를 정량하고 ICP-MS 분석 결과와 비교하였다.

• 분석과학
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• 제10권1호
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• pp.35-42
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• 1997

Barium titanate 및 PZT와 같은 세라믹 축전물질의 분석을 위해 고압 산분해법을 이용한 시료 전처리 기술을 연구하였다. 질산이나 증류수를 첨가하고 염산의 농도를 변화시키면서, 이들 시료의 정량분석을 유도결합 플라즈마 방출분광법에 의해 수행하였다. 분석 결과를 보면 Ba, Mn, Zn, Si 등 대부분의 원소들은 염산의 농도에 영향을 받지 않으나, Nb와 Zr은 이에 민감한 것으로 밝혀졌다. 그러나 분해시간은 상대적으로 분석 결과에 거의 영향을 미치지 않았다. Nb의 경우에는 가장 좋은 분석 결과를 얻기 위해 염산과 증류수의 비가 3:1(v / v) 보다는 더 진해야 함을 알았다. 또한 Pb의 분석에 있어서 염산과 질산의 혼산을 사용하는 경우보다 붉은 염산만을 사용하였을 경우에 더 좋은 분석 결과를 나타내었다.

• 분석과학
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• 제8권4호
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• pp.807-814
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• 1995

Accurate measurements of ozone precursors are required to understand the process and extent of ozone formation in rural and urban areas. Nonmethane hydrocarbons (NMHCs) have been identified as important ozone precursors. Identification and quantification of NMHCs are difficult because of the large number present and the wide molecular weight range encountered in typical air samples. A major plan of the research team of the Climate and Air Quality Taiwan Station (CATs) was the measurement of atmospheric nonmethane hydrocarbons. An analytical method has been development for the analysis of the individual nonmethane hydrocarbons in ambient air at ppb (v) and subppb(v) levels. The whole ambient air samples were collected in canisters and analyzed by GC-FID with $Al_2O_3$/KCl PLOT column. Our targeted for quantitative analysis 43 compounds that may be substantial contributors to ozone formation. The retention indices and molar response factors of some commercially available $C_2{\sim}C_{10}$ hydrocarbons were determined and used to identify and quantify air samples. A quality assurance program was instituted to ensure that good measurements were made by participating in the International Nonmethane Hydrocarbon Intercomparison Experiments (NOMHICE).

• 생약학회지
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• 제37권1호통권144호
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• pp.33-36
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• 2006

The quantitative analytical method for the content of dioscin in Dioscorea rhizoma using a high performance liquid chromatography(HPLC) system was established for its quality control. After extracting Discorea rhizoma flour with ethanol, dioscin was separated though an ODS column with a flow rate of 1.0ml/min of acetonnitril-methanol-0.01 M phosphate buffer (pH 5.0)(6:3:1, v/v%), and the amount of dioscin was detected at 210nm. Relation time of dioscin in HPLC chromatogram were about $7.45{\pm}0.34\;min$ and calibration curve showed good linearity at concentrations from 0.1 to 2.0 mg/ml of dioscin. When 5 commercial Dioscorea rhizoma flours were analyzed by HPLC, the peak for dioscin was well separated from others in ethanol extract of Dioscorea rhizoma, and the amount of dioscin was in the range from 0.076 to 0.142(w/w)%.

• 분석과학
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• 제36권1호
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• pp.32-43
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• 2023

This study reports for the first time about a stability indicating RP-HPLC method for qualitative and quantitative determination of acalabrutinib in bulk and dosage form and in presence its impurities 1, 2 and 3. The chromatographic separation was carried on Zorbax XDB-C18 (250×4.6 mm; 5 µ id) as stationary phase, Phosphate buffer pH 6.4 and methanol 80:20 (v/v) as mobile phase at a flow rate of 1.0 mL/min, UV detection was carried at wavelength of 238 nm and the analysis was completed with a run time of 15 min. In these conditions the retention time of acalabrutinib and its impurities 1, 2 and 3 was observed to be 3.50, 4.83, 8.40 and 9.93 min respectively. The method was validated for system suitability, range of analysis, precision, specificity, stability and robustness. Spiked recovery at 50 %, 100 % and 150 % was carried for both standard and impurities and the acceptable % recovery of 98-102 was observed for acalabrutinib and both impurities studied and the % RSD in each spiked level was found to be less than 2. Stability tests were done through exposure of the analyte solution to five different stress conditions i.e expose to 1N hydrochloric acid, 1 N sodium hydroxide, 3 % peroxide, 80 ℃ temperature and UV radiation at 254 nm. In all the degradation condition, standard drug acalabrutinib was detected along with both the impurities studied and the degradation products were successfully separated. In the formulation analysis there is no other chromatographic detection of other impurities and formulation excipients. Hence the developed method was found to be suitable for the quantification of acalabrutinib and can separate and analyse impurities 1 and 2.