• Asian-Australasian Journal of Animal Sciences
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• 제13권11호
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• pp.1604-1608
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• 2000

Penicillin antibiotics such as penicillin G, ampicillin and amoxicillin have been widely used in the pig industry to control salmonellosis, bacterial pneumonia, and urinary tract infections. Extensive use of antibiotics in veterinary clinics has resulted in tissue residues and bacterial resistance. To prevent unwanted drug residues entering the human food chain, extensive control measures have been established by both government authorities and industries. The demands for reliable, simple, sensitive, rapid and low-cost methods for residue analysis of foods are increasing. In this study, we established a rapid prediction test for the detection of pigs with unacceptable tissue residues of penicillins. The recommended therapeutic doses of three penicillins, penillin G (withdrawal time, 7 days), ampicillin (withdrawal time, 7 days) and amoxicillin (withdrawal time, 14 days), were administered to three groups of 20 pigs each. Blood was sampled before drug administration and during the withdrawal period. The concentration of penicillins in plasma, determined by a semi-quantitative ELISA, were compared to that of internal standard, 4 ppb, which corresponded to the Maximum Residue Limit in milk. The absorbance ratio of internal standard to sample (B/Bs) was employed as an index to determine whether drug residues in pig tissues were negative or positive. That is, a B/Bs ratio less than 1 was considered residue positive, and larger than 1 negative. All 60 plasma samples from pigs were negative to three penicillins at pretreatment. Penicillin G could be detected in the plasma of the treated pigs until day 4 post-treatment and ampicillin until day 2, whereas amoxicillin could be detected until day 10 of its withdrawal period. The present study showed that the semi-quantitative ELISA could be easily adapted to detect residues of penicillin antibiotics (penicillin G, ampicillin and amoxicillin) in live pigs.

• 분석과학
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• 제30권6호
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• pp.319-328
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• 2017

The identification of explosive residues on specimens obtained from an explosion event is a crucial factor for assessing the cause of the explosion. In order to detect the components of explosives, the explosive residues deposited on surfaces are commonly extracted using swabbing materials pre-wetted with an organic solvent. The residues are then analyzed with analytical instruments such as LC/MS and CE/MS. Most conventionally used swabbing media such as cotton swabs or cotton tip swabs seem unsuitable for extracting explosive residues from the surface of a large area of clothes because the swabbing materials tend to be damaged easily, and because only a relatively small amount of explosives is collected. To overcome these problems, we have introduced a novel wiper ($215{\times}210mm$, single layer, Yuhan-Kimberly, Republic of Korea) as a swabbing material to recover representative organic explosives, namely, TNT, RDX, tetryl, HMX, PETN, and NG, from a large area of clothes. Different sides of the wiper, which was folded in half five times, was used to swab the surface of a clothing. We compared this novel wiper with a cotton swab and a cotton tip swab in terms of the recovery efficiency for the aforementioned organic explosives by pre-wetting with methanol, acetone, and acetonitrile, respectively. We identified that this novel wiper collected a significantly higher amount of organic explosive residues than a cotton swab or a cotton tip swab when using methanol as an extracting solvent.

• 농약과학회지
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• 제14권1호
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• pp.16-20
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• 2010

Thiosultap은 중국에서 사용되고 있는 nereistoxin계 살충제로 국내에는 등록되지 않아 중국산 농산물 수입시 잔류 농약 안전관리를 위한 시험법 마련이 시급한 실정이다. 이에 본 연구에서는 현미 중 thiosultap을 염기조건에서 nereistoxin으로 유도체화하여 GC-FPD로 분석하는 시험법을 개발하였다. 산염기 분배를 이용한 정제 조건을 확립하였으며, 확립된 시험법에 의한 정량한계와 직선성을 측정한 결과 각각 0.05 mg $kg^{-1}$과 0.995$(r^2)$이었다. 무처리 현미에 thiosultap 0.5와 2.5 mg $kg^{-1}$을 처리하여 회수율을 측정한 결과는 $96.1{\pm}7.9\sim100.8{\pm}6.1%$로 양호한 결과를 나타내었다.

• 대한수의학회지
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• 제56권4호
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• pp.233-239
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• 2016

This study was conducted to analyze penicillin G (PEG), streptomycin (STR) and neomycin (NEO) residues in milk of healthy lactating cows. Milk samples were collected from all four quarters of 12 dairy cows 2−7 days after intramammary infusions of an ointment containing PEG, STR and NEO once (n = 4; group I) or twice (n = 4, group II) daily. Ultra-performance liquid chromatography coupled with electrospray tandem mass spectrometry was used to determine the antibiotic residues in the samples. The correlation coefficient ($r^2$) of the calibration curves for all antibiotics was > 0.999 and the limits of detection and quantification were $0.002-0.005{\mu}g/mL$ and $0.007-0.02{\mu}g/mL$, respectively. Recovery rates were ranged from 75.5 to 92.3%. In group I, PEG, STR and NEO residues were detected in milk at 2, 3 and 2 days post-treatment, respectively, which were below the maximum residue limit (MRL). In group II, PEG, STR and NEO residues were detected in milk at 2, 3 and 3 days post-treatment, respectively, which were bellow the MRL. These results suggest that a 3-day for milk withdrawal period after the ointment treatment might be sufficient for reduction of the antibiotic residues below the MRL.

• BMB Reports
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• 제37권2호
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• pp.254-259
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• 2004

The wild-type and temperature-sensitive (ts) repressor genes were cloned from the temperate mycobacteriophage L1 and its mutant L1cIts391, respectively. A sequencing analysis revealed that the $131^{st}$ proline residue of the wild-type repressor was changed to leucine in the ts mutant repressor. The 100% identity that was discovered between the two DNA regions of phages L1 and L5, carrying the same sets of genes including their repressor genes, strengthened the speculation that L1 is a minor variant of phage L5 or vice versa. A comparative analysis of the repressor proteins of different mycobacteriophages suggests that the mycobacteriophage-specific repressor proteins constitute a new family of repressors, which were possibly evolved from a common ancestor. Alignment of the mycobacteriophage-specific repressor proteins showed at least 7 blocks (designated I-VII) that carried 3-8 identical amino acid residues. The amino acid residues of blocks V, VI, and some residues downstream to block VI are crucial for the function of the L1 (or L5) repressor. Blocks I and II possibly form the turn and helix 2 regions of the HTH motif of the repressor. Block IV in the L1 repressor is part of the most charged region encompassing amino acid residues 72-92, which flanks the putative N-terminal basic (residues 1-71) and C-terminal acidic (residues 93-183) domains of L1 repressor.

• BMB Reports
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• 제33권6호
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• pp.531-536
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• 2000

Tropomyosin (TM) is an important actin binding protein involved in regulation of muscle contraction. Unacetylated striated tropomyosin failed to bind to actin whereas unacetylated smooth tropomyosin bound well to actin. It has been demonstrated that high actin affinity of unacetylated ${\alpha}-tropomyosin$ was ascribed to the carboxyl terminal amino acid residues. In order to define the role of the carboxyl terminal residues of tropomyosin molecule on actin binding, two mutant tropomyosins were constructed. TM11 is identical to the striated tropomyosin except that the carboxyl terminal last three amino acids was replaced with $^{282}NNM^{284}$ whereas in TM14 $^{276}HA^{277}$ was substituted with smooth specific $^{276}QT^{277}$. TM11 and TM14 were overproduced in Escherichia coli and analyzed for actin affinity. The apparent binding constants (Kapp) of unacetylated tropomyosins were $2.2{\times}10^6M^{-1}$ for sm9, $1.03{\times}10^6M^{-1}$ for TM14, $0.19{\times}10^6M^{-1}$ for TM11, $>0.1{\times}10^6M^{-1}$ for striated, respectively. This result indicated that higher actin affinity of the unacetylated smooth tropomyosin was primarily attributed to the presence of QT residues in the smooth sequence. In case of the Ala-Ser (AS) dipeptide extension of the amino terminus of tropomyosin, Kapp were $21.1{\times}10^6M^{-1}$ for AS-sm9, $8.0{\times}10^6M^{-1}$ for AS-11, $4.7{\times}10^6M^{-1}$ for AS-14, $3.8{\times}10^6M^{-1}$ for AS-striated. AS-TM11 showed considerably higher actin affinity than AS-TM14, implying that interaction of Ala-Ser of the amino terminus with the carboxyl terminal residues. Since Kapp of AS-TM11 was significantly lower than that of AS-sm9, the presence of QT might be required for restoration of high actin affinity of the smooth ${\alpha}-tropomyosin$. These results suggested that the carboxyl terminal amino acid residues Glutamine275-Threonine276 are important for actin affinity of the recombinant smooth ${\alpha}-tropomyosin$, particularly of unacetylated smooth ${\alpha}-tropomyosin$.

• 한국균학회지
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• 제26권1호통권84호
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• pp.47-50
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• 1998

농산부산물첨가배지 개발로서 이화학적 특성은 콩비지첨가구에서 유기물, 질소, 탄소 함량이 높았으며 전처리구의 pH, 유기물, 질소, 탄소 함량은 버섯 생육시 적합한 것으로 판단되었다. 애느타리 관행재배시 병당(850cc)에서 갓의수 20개 72g에 비하여 콩비지 10% 첨가구는 갓의 수 12개 수량 77g으로 7% 증수, 귤껍질 10% 첨가구는 갓의 수 21개 수량 11% 증수되었다. 버들송이 관행재배시 병당 (850cc) 수량 98g 대비 한약박을 제외한 모든 농산부산물 첨가해서 증수되었으나 그중 콩비지 10% 첨가구가 수량 113g으로 15% 증수되었다. 저비용 고효율 농산부산물 버섯 배지개발로써 농가경영비 절감과 고품질 버섯 생산으로 농가소득에 기여할 것이다.

• 자원리싸이클링
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• 제9권3호
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• pp.22-28
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• 2000

아연재련전사로부터 갈륨을 회수하기 위하여 NaOH용액을 사용한 알칼리 침출실험을 수행하였다. 실험결과 아연질산을 NaOH용액으로 알칼리 침출할 경우 주로 침출되는 원소는 Zn, K 및 Si 등이며, Fe를 비롯한 여러 base metal들은 극히 미량만이 침출되기 때문에 용매추출 공정을 통해 용이하게 갈륨을 정제할 수 있다. 한편 알칼리 침출의 특징은 알칼리 농도가 증가할수록 그리고 광액농도가 낮을수록 갈륨의 침출율이 증가하며, 특히 침출에 앞서 아연잔사를 물로 세척하여 용해성 아연화합물을 미리 제거하면 알칼리 소모량을 상당히 줄일 수 있는 것으로 나타났다. 대체로 갈륨의 적정 침출조건은 아연잔사를 물로 세척하여 용해성 아연화합물을 미리 제거하고 광액농도 333g/L NaOH 농도 1~1.25 M/L로 하여 상온$25^{\circ}C$에서 2시간 정도 침출하는 것이 효과적이며, 이 경우 약 80%이상의 갈륨을 회수 할 수있다.

• 미생물학회지
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• 제47권4호
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• pp.302-307
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• 2011

A. nidulans chitin deacetylase를 자가분해 용액으로부터 소수성 상호작용 컬럼 크로마토그래피와 이온 교환 컬럼 크로마토그래피를 통해 순수 분리하였다. 효소 활성에 관여하는 아미노산을 분석하기 위해 효소 단백질과 특정 아미노산 잔기에 작용하는 화학 수식제를 반응시켜 효소를 화학 수식하였다. histidine 잔기가 화학 수식된 효소는 효소활성을 100% 상실하였으며, arginine의 잔기 혹은 tyrosine 잔기는 100 ${\mu}M$보다 높은 농도의 수식제로 화학수식 되었을 때 효소활성이 감소하였다. Aspartic acid 혹은 glutamic acid의 carboxyl group 잔기의 화학수식은 효소활성의 상대적으로 작은감소를 나타냈다. 이것은 산성 아미노산의 잔기가 화학 촉매 반응에 직접 관여하지 않았거나 혹은 산성 아미노산 잔기는 효소단백질의 전반적인 구조에 영향을 미친다는 것을 추론할 수 있다. 이러한 결과는 효소 단백질의 촉매활성에 histidine, tyrosine 및 arginine 잔기가 중요한 역할을 담당하는 것을 의미한다.

• 한국축산식품학회지
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• 제43권5호
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• pp.914-937
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• 2023

The objective of this study was to establish a multi-residue quantitative method for the analysis of anthelmintic and antiprotozoal drugs in various livestock products (beef, pork, and chicken) using ultra-high-performance liquid chromatography-tandem mass spectrometry. Each compound performed validation at three different levels i.e., 0.5, 1, and 2× the maximum residue limit according to the CODEX guidelines (CAC/GL 71-2009). This study was conducted according to the modified quick, easy, cheap, effective, rugged, and safe procedure. The matrix-matched calibrations gave correlation coefficients >0.98, and the obtained recoveries were in the range of 60.2%-119.9%, with coefficients of variation ≤32.0%. Furthermore, the detection and quantification limits of the method were in the ranges of 0.03-3.2 and 0.1-9.7 ㎍/kg, respectively. Moreover, a survey of residual anthelmintic and antiprotozoal drugs was also carried out in 30 samples of beef, pork, and chicken collected in Korea. Toltrazuril sulfone was detected in all three samples. Thus, our results indicated that the developed method is suitable for determining the anthelmintic and antiprotozoal drug contents in livestock products.