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On-site rapid detection of multiple pesticide residues in tea leaves by lateral flow immunoassay
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作者 Junxia Gao Tianyi Zhang +7 位作者 Yihua Fang Ying Zhao Mei Yang Li Zhao Ye Li Jun Huang Guonian Zhu Yirong Guo 《Journal of Pharmaceutical Analysis》 SCIE CAS CSCD 2024年第2期276-283,共8页
The application of pesticides (mostly insecticides and fungicides) during the tea-planting process will undoubtedly increase the dietary risk associated with drinking tea. Thus, it is necessary to ascertain whether pe... The application of pesticides (mostly insecticides and fungicides) during the tea-planting process will undoubtedly increase the dietary risk associated with drinking tea. Thus, it is necessary to ascertain whether pesticide residues in tea products exceed the maximum residue limits. However, the complex matrices present in tea samples comprise a major challenge in the analytical detection of pesticide residues. In this study, nine types of lateral flow immunochromatographic strips (LFICSs) were developed to detect the pesticides of interest (fenpropathrin, chlorpyrifos, imidacloprid, thiamethoxam, acetamiprid, carbendazim, chlorothalonil, pyraclostrobin, and iprodione). To reduce the interference of tea substrates on the assay sensitivity, the pretreatment conditions for tea samples, including the extraction solvent, extraction time, and purification agent, were optimized for the simultaneous detection of these pesticides. The entire testing procedure (including pretreatment and detection) could be completed within 30 min. The detected results of authentic tea samples were confirmed by ultra-performance liquid chromatography-tandem mass spectrometry (UPLC-MS/MS), which suggest that the LFICS coupled with sample rapid pretreatment can be used for on-site rapid screening of the target pesticide in tea products prior to their market release. 展开更多
关键词 Lateral flow immunoassay rapid detection Pesticide multi-residue Tea matrix Sample rapid pretreatment
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Rapid Detection of Somatic Cell Count Based on Hybrid Variable Selection Method
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作者 Shen Weizheng Cui Xiang +6 位作者 Wang Yan Nie Debao Zhang Qinggang Zheng Wei Sun Jian Yang Xin Dai Baisheng 《Journal of Northeast Agricultural University(English Edition)》 CAS 2024年第3期59-73,共15页
Somatic cell count detection is the daily work of dairy farms to monitor the health of cows.The feasibility of applying near-infrared spectroscopy to somatic cell count detection was researched in this paper.Milk samp... Somatic cell count detection is the daily work of dairy farms to monitor the health of cows.The feasibility of applying near-infrared spectroscopy to somatic cell count detection was researched in this paper.Milk samples with different somatic cell counts were collected and preprocessing methods were studied.Variable selection algorithm based on hybrid strategy and modelling method based on ensemble learning were explored for somatic cell count detection.Detection model was used to diagnose subclinical mastitis and the results showed that near-infrared spectroscopy could be a tool to realize rapid detection of somatic cell count in milk. 展开更多
关键词 near-infrared spectroscopy somatic cell count MASTITIS rapid detection
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Establishment of High-sensitivity Rapid Fluorescence Quantitative Detection Method for Antibody against Peste des Petits Ruminants Virus
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作者 Zhao LIU Bo LIU +3 位作者 Zhida LIN Hang SUN Yu SUN Xiaohui SONG 《Agricultural Biotechnology》 2024年第5期22-27,共6页
[Objectives]This study was conducted to establish a rapid quantitative method for detecting antibody against Peste des Petits Ruminants Virus(PPR V)in sheep serum.[Methods]Soluble N protein and NH fusion protein were ... [Objectives]This study was conducted to establish a rapid quantitative method for detecting antibody against Peste des Petits Ruminants Virus(PPR V)in sheep serum.[Methods]Soluble N protein and NH fusion protein were obtained in Escherichia coli prokaryotic expression system by optimizing codons and expression conditions of E.coli.Furthermore,based on the purified soluble N protein and NH fusion protein,a high-sensitivity fluorescence immunoassay kit for detecting the antibody against PPR V was established.[Results]The method could quickly and quantitatively detect PPR V antibody in sheep serum,with high sensitivity and specificity,without any cross reaction to other related sheep pathogens.The intra-batch and inter-batch coefficients of variation were less than 10%and 15%,respectively,and the method had good repeatability.Through detection on 292 clinical serum samples,it was compared with the French IDVET competitive ELISA kit,and the coincidence rate of the two methods reached 93.84%.Compared with the serum neutralization test,the detected titer value of the high-sensitivity rapid fluorescence quantitative detection method was basically consistent with the tilter value obtained by the neutralization test on the standard positive serum(provided by the WOAH Brucellosis Reference Laboratory of France).[Conclusions]This method can realize rapid quantitative detection of PPR V antibody on site,and has high practical value and popularization value. 展开更多
关键词 Peste des Petits Ruminants N protein NH fusion protein Soluble expression and purification rapid quantitative detection
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Establishment and application of a rapid visualization method for detecting Vibrio parahaemolyticus nucleic acid
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作者 Yachao Hou Xinping Liu +7 位作者 Ya’nan Wang Liang Guo Lvying Wu Wenrong Xia Yongqi Zhao Weiwei Xing Jin Chen Changguo Chen 《Infectious Medicine》 2024年第2期55-65,共11页
Background:Swift and accurate detection of Vibrio parahaemolyticus,which is a prominent causative pathogen associated with seafood contamination,is required to effectively combat foodborne disease and wound infections... Background:Swift and accurate detection of Vibrio parahaemolyticus,which is a prominent causative pathogen associated with seafood contamination,is required to effectively combat foodborne disease and wound infections.The toxR gene is relatively conserved within V.parahaemolyticus and is primarily involved in the expression and regulation of virulence genes with a notable degree of specificity.The aim of this study was to develop a rapid,simple,and constant temperature detection method for V.parahaemolyticus in clinical and nonspecialized laboratory settings.Methods:In this study,specific primers and CRISPR RNA were used to target the toxR gene to construct a reaction system that combines recombinase polymerase amplification(RPA)with CRISPR‒Cas13a.The whole-genome DNA of the sample was extracted by self-prepared sodium dodecyl sulphate(SDS)nucleic acid rapid extraction reagent,and visual interpretation of the detection results was performed by lateral flow dipsticks(LFDs).Results:The specificity of the RPA-CRISPR/Cas13a-LFD method was validated using V.parahaemolyticus strain ATCC-17802 and six other non-parahaemolytic Vibrio species.The results demonstrated a specificity of 100%.Additionally,the genomic DNA of V.parahaemolyticus was serially diluted and analysed,with a minimum detectable limit of 1 copy/μL for this method,which was greater than that of the TaqMan-qPCR method(10^(2) copies/μL).The established methods were successfully applied to detect wild-type V.parahaemolyticus,yielding results consistent with those of TaqMan-qPCR and MALDI-TOF MS mass spectrometry identification.Finally,the established RPA-CRISPR/Cas13a-LFD method was applied to whole blood specimens from mice infected with V.parahaemolyticus,and the detection rate of V.parahaemolyticus by this method was consistent with that of the conventional PCR method.Conclusions:In this study,we describe an RPA-CRISPR/Cas13a detection method that specifically targets the toxR gene and offers advantages such as simplicity,rapidity,high specificity,and visual interpretation.This method serves as a valuable tool for the prompt detection of V.parahaemolyticus in nonspecialized laboratory settings. 展开更多
关键词 Vibrio parahaemolyticus RPA CRISPR/Cas13a rapid detection Visual approach
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Recent Advances in the Rapid Detection and Performance Evaluation Methods of Detergent Additives for Gasoline
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作者 Zhi Wanwan Li Na +2 位作者 Zhu Zhongpeng Li Yan Guo Xin 《China Petroleum Processing & Petrochemical Technology》 SCIE CAS CSCD 2023年第2期165-176,共12页
Although detergent additives for gasoline have been widely commercialized,their formulas are often kept confidential and there is still no standardized method for quickly detecting the main active ingredients and eval... Although detergent additives for gasoline have been widely commercialized,their formulas are often kept confidential and there is still no standardized method for quickly detecting the main active ingredients and evaluating their effectiveness,which makes their regulation difficult.An overview of the current state of the development and application of detergent additives for gasoline in China and other regions,as well as a review of the rapid detection and performance evaluation methods available for analyzing detergent additives are given herein.The review focuses on the convenience,cost,efficiency,and feasibility of on-site detection and the evaluation of various methods,and also looks into future research directions,such as detecting and evaluating detergent additives in ethanol gasoline and with advanced engine technologies. 展开更多
关键词 GASOLINE detergent additives DEPOSITS rapid detection performance evaluation
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Filtration assisted pretreatment for rapid enrichment and accurate detection of Salmonella in vegetables
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作者 Bin Li Hanling Wang +5 位作者 Jianguo Xu Wei Qu Li Yao Bangben Yao Chao Yan Wei Chen 《Food Science and Human Wellness》 SCIE CSCD 2023年第4期1167-1173,共7页
Rapid detection of target foodborne pathogens plays more and more significant roles in food safety,which requires the efficiency,sensitivity,and accuracy.In this research,we proposed a new st rategy of isothermal-mole... Rapid detection of target foodborne pathogens plays more and more significant roles in food safety,which requires the efficiency,sensitivity,and accuracy.In this research,we proposed a new st rategy of isothermal-molecular-amplification integrated with lateral-flow-strip for rapid detection of Salmonella without traditional enrichment-culture.Th e designed syringe-assisted-filtration can contribute to simultaneous collection and concentration of target bacterium from vegetable samples in just 3 min,resolving the drawbacks of traditional random sampling protocols.After simple and convenient ultrasonication,samples can be directly amplified at 39℃ in 25 min and the amplicons are qualitatively and quantitatively analyzed with the designed lateral-flow-strip in 5 min.Finally,satisfied results have been achieved within 40 min,which greatly improve the efficiency while the accuracy is also guaranteed.Furthermore,all detection steps can be completed under instrument-free conditions.This method will hold great promise for target pathogen detection in the resource-limited district,or for emergency on-site identification. 展开更多
关键词 VEGETABLES SALMONELLA Filtration enrichment Culture-free detection Enzymatic recombinase amplification(ERA) Lateral flow strip(LFS) rapid detection Food safety
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Establishment of a rapid detection method of Ureaplasma urealyticum based on recombinant polymerase amplification
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作者 He-Hui Yang Yi-Chao Wang Jiao-Gui Xie 《Life Research》 2023年第4期34-41,共8页
Ureaplasma urealyticum(UU),is one of the most vital pathogens causing genitourinary tract infections of the body,and it can result in poor maternal and perinatal outcomes.The aim of this study was to establish a metho... Ureaplasma urealyticum(UU),is one of the most vital pathogens causing genitourinary tract infections of the body,and it can result in poor maternal and perinatal outcomes.The aim of this study was to establish a method to detect Ureaplasma urealyticum based on recombinant polymerase amplification(RPA)technique.Specific primers and probes were designed according to the 16sRNA gene sequence of Ureaplasma urealyticum.Six pathogens were detected for real-time fluorescence RPA specificity verification,including Mycoplasma hominis(MH),Chlamydia trachomatis(CT),Neisseria gonorrhoeae(NG),Staphylococcus aureus,Escherichia coli,and Lactobacillus vaginalis.The sensitivity of the method was performed by gradient dilution of the extracted template.A total of 60 clinical samples were detected by the established real-time fluorescence RPA.Detection of Ureaplasma urealyticum can be completed within 20 minutes at 39°C using established RPA method.The minimum detection limit of Ureaplasma urealyticum by real-time fluorescence RPA was 3 pg.The evaluation of 60 clinical samples proved that RPA method was feasible.A high specificity,sensitivity,simplicity and rapidity method for Ureaplasma urealyticum detection was successfully established based on the real-time fluorescence RPA method. 展开更多
关键词 Ureaplasma urealyticum recombinase polymerase amplification(RPA) rapid detection fluorescence probe
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A Rapid and Simple Method for the Detection of Rice Dwarf Virus by Aqueous Extract 被引量:2
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作者 许曼琳 杨金广 《Agricultural Science & Technology》 CAS 2010年第3期98-100,共3页
Rice dwarf disease caused by rice dwarf virus (RDV) is one of the major rice virus diseases in China,which widely distributes in the rice area of China.A simple and rapid method for detection of RDV in rice plants a... Rice dwarf disease caused by rice dwarf virus (RDV) is one of the major rice virus diseases in China,which widely distributes in the rice area of China.A simple and rapid method for detection of RDV in rice plants and Nephotettix cincticeps was investigated in this study,and the whole detection only lasted for 20 min.After diseased leaves of rice (10 mg) and leaves of Nephotettix cincticeps (10 mg) both infected by RDV were ground by sterile water (100 μl),the supernatant was analyzed by 1% agarose gel electrophoresis to steadily detect five specific electrophoretic bands with 1 000 bp to 5 000 bp.However,there was no electrophoretic band in the healthy rice leaves and aqueous extract of non-viruliferous N.cincticeps.Therefore,this method was more rapid and simple to detect RDV in rice plants and Nephotettix cincticeps,which avoided expensive reagents and tedious steps of conventional serological testing and molecular detection (RT-PCR and Western-blot). 展开更多
关键词 Rice dwarf virus Aqueous extract rapid detection
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The Application of Reverse Transcription-loop-mediated Isothermal Amplification for the Rapid Detection of Maize Chlorotic Dwarf Virus
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作者 徐颖 张峰 +1 位作者 于莹 邱志君 《Agricultural Science & Technology》 CAS 2017年第12期2450-2453,共4页
Maize chlorotic dwarf virus (MCDV) is a quarantine pest as approved by Chinese government. A rapid, sensitive and specific MCDV detection method using reverse transcription-loop-mediated isothermal amplification (R... Maize chlorotic dwarf virus (MCDV) is a quarantine pest as approved by Chinese government. A rapid, sensitive and specific MCDV detection method using reverse transcription-loop-mediated isothermal amplification (RT-LAMP) was estab- lished in this study. Based on the sequence of MCDV coat protein coding gene, specific primers were designed and similar sensitivities were observed between RT- LAMP and RT-PCR, except that RT-LAMP was quicker, and the reaction could be finished within 1 h. In addition, the presence or absence of the fluorescent display in daylight allows naked easy detection of the amplification of MCDV genomic RNA using calcein. The RT-LAMP assay was applied successfully to detect MCDV in maize seeds, and the result by the addition of calcein was consistent with the result detected by the real time turbidimeter. 展开更多
关键词 Maize chlorotic dwarf virus (MCDV) Reverse transcription loop-mediatedisothermal amplification (RT-LAMP) rapid detection
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Luciferase reporter phage phAE85 for rapid detection of rifampicin resistance in clinical isolates of Mycobacterium tuberculosis 被引量:4
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作者 Gomathi Sivaramakrishnan Balaji Subramanyam +1 位作者 Ponnuraja C Vanaja Kumar 《Asian Pacific Journal of Tropical Medicine》 SCIE CAS 2013年第9期728-731,共4页
Objective:To evaluate luciferase reporter phage(LRP)phAE85 in rapid detection of rifampicin resistance in a region where TB is endemic.Methods:One hundred and ninety primary isolates on Lowenstein-Jensen medium were t... Objective:To evaluate luciferase reporter phage(LRP)phAE85 in rapid detection of rifampicin resistance in a region where TB is endemic.Methods:One hundred and ninety primary isolates on Lowenstein-Jensen medium were tested.Middlebrook 7H9 complete medium with and without rifampicin at 2μg/mL was inoculated with standard inoculum from suspensions of the clinical isolate.After incubation for 72 h,LRP was added.Following 4 h of further incubation,light output from both control and test was measured as relative light units.Strains exhibiting a reduction of less than 50%relative light units in the drug containing vial compared to control were classified as resistant.Results were compared with the conventional minimum inhibitory concentration method(MIC)of drug susceptibility testing.Results:The two methods showed high level of agreement of 97%(CI 0.94,0.99)and P value was 0.000 1.The sensitivity and specificity of LRP assay for detection of rifampicin resistance were 91%h(CI 0.75,0.98)and 99ct(CI0.95,1.00)respectively.Time to detection of resistance by LRP assay was 3 d in comparison with 28 d by the minimum inhibitory concentration method.Conclusions:LRP assay with phAE85 is 99%specific,91%sensitive and is highly reproducible.Thus the assay offers a simple procedure for drug sensitivity testing,within die scope of semi-automation. 展开更多
关键词 MYCOBACTERIUM TUBERCULOSIS RIFAMPICIN RESISTANCE rapid detection
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Study on Colloidal Gold Immunochromatography Assay for Rapid Detection of Spectinomycin 被引量:3
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作者 Zhaoqin WANG Yuping WAN +5 位作者 Xiaosheng WU Yu ZHANG Fangfang JIA Guangyao HAN Zhengxue PENG Fangyang HE 《Agricultural Biotechnology》 CAS 2019年第1期188-189,193,共3页
[Objectives] This study was conducted to establish a rapid detection method for spectinomycin in pork,chicken,fish,shrimp flesh and water.[Methods]A test strip for rapid detection of spectinomycin in milk was develope... [Objectives] This study was conducted to establish a rapid detection method for spectinomycin in pork,chicken,fish,shrimp flesh and water.[Methods]A test strip for rapid detection of spectinomycin in milk was developed by colloidal gold immunochromatography assay. [Results]The test strip had a detection limit of 50 μg/kg to milk with a detection time of 15 min,and the false positive rate and false negative rate were both 0. [Conclusions]The method is accurate,simple,reliable and convenient,and is suitable for rapid on-site spectinomycin detection. 展开更多
关键词 SPECTINOMYCIN Gold IMMUNOCHROMATOGRAPHY ASSAY rapid test STRIP rapid detection
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Enzyme Inhibition Rate Method for Rapid Detection of Organophosphorus and Carbamate Pesticides in Cowpea 被引量:4
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作者 Mai Changqing Chen Sheng Chen Yan 《Plant Diseases and Pests》 CAS 2017年第4期30-32,共3页
[Objectives ] The paper was to explore enzyme inhibition rate method for rapid detection of organophosphorus and carbamate pesticides in cowpea. [ Methods ] Acetylcholinesterase (ACHE) was added to cowpea extract, t... [Objectives ] The paper was to explore enzyme inhibition rate method for rapid detection of organophosphorus and carbamate pesticides in cowpea. [ Methods ] Acetylcholinesterase (ACHE) was added to cowpea extract, to determine the inhibition rate of extract against enzyme. The influences of different sampiing methods and sampling parts on detection results were compared. [ Results] The positive rate of standard sampling was 18.18% higher than that of non-stand- ard sampling, and the positive rate of samples collected from cowpea tail was 16.67% higher than that collected from other parts. [ Condmions] Enzyme inhibi- tion rate method is suitable for rapid detection of organophosphorus and carbamate pesticides in cowpea. 展开更多
关键词 Enzyme inhibition rate method Organophosphorus pesticide Carbamate pesticide COWPEA rapid detection
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In vitro Selection of DNA Aptamers and Fluorescence-Based Recognition for Rapid Detection Listeria monocytogenes 被引量:4
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作者 LIU Guo-qing LIAN Ying-qi +5 位作者 GAO Chao YU Xiao-feng ZHU Ming ZONG Kai CHEN Xue-jiao YAN Yi 《Journal of Integrative Agriculture》 SCIE CAS CSCD 2014年第5期1121-1129,共9页
Aptamers are specific nucleic acid sequences that can bind to a wide range of nucleic acid and non-nucleic acid targets with high affinity and specificity. Nucleic acid aptamers are selected in vitro from single stran... Aptamers are specific nucleic acid sequences that can bind to a wide range of nucleic acid and non-nucleic acid targets with high affinity and specificity. Nucleic acid aptamers are selected in vitro from single stranded DNA or RNA ligands containing random sequences of up to a few hundred nucleotides. Systematic evolution of ligands by exponential enrichment (SELEX) was used to select and PCR amplify DNA sequences (aptamers) capable of binding to and detecting Listeria monocytogenes, one of the major food-borne pathogens. A simplified affinity separation approach was employed, in which L. monocytogenes in exponential (log) phase of growth was used as the separation target. A fluorescently-labeled aptamer assay scheme was devised for detecting L. monoeytogenes. This report described a novel approach to the detection of L. monocytogenes using DNA aptamers. Aptamers were developed by nine rounds of SELEX. A high affinity aptamer was successfully selected from the initial random DNA pool, and its secondary structure was also investigated. One of aptamers named e01 with the highest affinity was further tested in aptamer-peroxidase and aptamer-fluorescence staining protocols. This study has proved the principle that the whole-cell SELEX could be a promising technique to design aptamer-based molecular probes for dectection of pathogenic microorganisms without tedious isolation and purification of complex markers or targets. 展开更多
关键词 aptamers systematic evolution of ligands by exponential enrichment (SELEX) Listeria monocytogenes rapid detection
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Rapid detection of Pseudomonas aeruginosa by cross priming amplification 被引量:4
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作者 XIANG Yong YAN Ling +3 位作者 ZHENG Xiao-cui LI Li-zhen LIU Peng CAO Wei-sheng 《Journal of Integrative Agriculture》 SCIE CAS CSCD 2020年第10期2523-2529,共7页
Pseudomonas aeruginosa(PA)is an opportunistic pathogen of humans and animals and a common source of nosocomial infections especially of the respiratory tract.Pseudomonas aeruginosa is also a major bacterial disease of... Pseudomonas aeruginosa(PA)is an opportunistic pathogen of humans and animals and a common source of nosocomial infections especially of the respiratory tract.Pseudomonas aeruginosa is also a major bacterial disease of poultry and in particular,eggs and newly hatched chicks.In this study,we developed a simple,accurate and rapid molecular detection method using cross priming amplification(CPA)with a nucleic acid test strip to detect P.aeruginosa.The assay efficiently amplified the target gene within 45 min at 62℃only using a simple water bath.The detection limit of the method was 1.18x 102 copiesμL^-1 for plasmid DNA and 4.4 CFU mL^-1 for bacteria in pure culture,and was 100 times more sensitive than conventional PCR.We screened 83 clinical samples from yellow-feather broiler breeder chickens and hospitalized/treated dogs and cats using CPA,PCR and traditional culture methods.The positive sample ratios were 15.3%(13/83)by CPA,13.3%(11/83)by PCR and 12.1%(10/83)by the culture method.The established CPA method has significant advantages for detecting P.aeruginosa.The method is easy to use and possesses high specificity and sensitivity without the requirements of complicated experimental equipment.The PA-CPA assay is especially fit for outdoor and primary medical units and is an ideal system for the rapid detection and monitoring of P.aeruginosa. 展开更多
关键词 Pseudomonas aeruginosa cross priming amplification isothermal amplification rapid detection detection method
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A Novel RT-LAMP Assay for Rapid and Simple Detection of Classical Swine Fever Virus 被引量:13
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作者 Lei CHEN Xue-zheng FAN Qin WANG Lu XU Qi-zu ZHAO Yuan-chen ZHOU Jun LIU Bo TANG Xing-qi ZOU 《Virologica Sinica》 SCIE CAS CSCD 2010年第1期59-64,共6页
A simple and rapid assay for the detection of Classical swine fever virus(CSFV)was established using reverse transcription loop-mediated isothermal amplification(RT-LAMP).This study describes the amplification of the ... A simple and rapid assay for the detection of Classical swine fever virus(CSFV)was established using reverse transcription loop-mediated isothermal amplification(RT-LAMP).This study describes the amplification of the genomic RNA of CSFV under isothermal conditions(63℃)within one hour,using a set of six primers(two outer primers,two inner primers and two loop primers).This RT-LAMP assay showed 100-fold higher sensitivity than the standard RT-PCR method and identified eighteen additional positive cases that were negative when tested by RT-PCR.This RT-LAMP was able to detect all the 13 strains of CSFV but not the BVDV.PRRSV.SIV. PRV-PCV,thus showed a good specificity.Products amplified by RT-LAMP can be visualized by agarose gel electrophoresis and in addition,either as a white precipitate at the bottom of the tube after a pulse spin or as a color change when dyed with SYBR Green I which are visible to the naked eye.Because RT-LAMP is low-cost and produces rapid results,it has the potential to be an excellent tool for CSFV surveillance in the field,especially in developing countries. 展开更多
关键词 Classical swine fever virus (CSFV) Reverse transcription loop-mediated isothermal amplification(RT-LAMP) rapid detection
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Deterioration mechanism and rapid detection of performances of an existing subgrade in southern China 被引量:7
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作者 ZHANG Jun-hui DING Le +1 位作者 ZHENG Jian-long GU Fan 《Journal of Central South University》 SCIE EI CAS CSCD 2020年第7期2134-2147,共14页
To relieve the increasing traffic load, many early built highways need to be widened or reconstructed. The rapid performance detection to existing subgrades is important to their reasonable evaluation and maximized ut... To relieve the increasing traffic load, many early built highways need to be widened or reconstructed. The rapid performance detection to existing subgrades is important to their reasonable evaluation and maximized utilization. Based on five kinds of soils taken from an existing highway in southern China, three commonly detecting methods were used to determine their moisture contents, compaction degrees and resilient moduli. The results showed that the measured moisture contents were greater than the design value, and the compaction degrees decreased sharply compared to the original ones. The moisture and heat exchange produced a decrease in the resilient modulus of plate loading test(PLT) from the standard 60 MPa down to 40 MPa. Afterwards, the portable falling weight deflectometer(PFWD) and dynamic cone penetrometer(DCP) were used to evaluate the subgrade performances. The measured PFWD moduli and the DCP penetration rates were correlated with the resilient moduli of PLT, deflections of the Beckman beam test, compaction degrees and moisture contents. The correlation analysis indicates that both of two methods are suitable in rapid detecting subgrade performances, but PFWD method is more recommended for it has higher accuracy and efficiency. 展开更多
关键词 humid and hot areas existing subgrade deterioration mechanism rapid detection portable falling weight deflectometer dynamic cone penetrometer
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Rapid Detection of Wheat Blast Pathogen Magnaporthe oryzae Triticum Pathotype Using Genome-Specific Primers and Cas12a-mediated Technology 被引量:7
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作者 Houxiang Kang Ye Peng +11 位作者 Kangyu Hua Yufei Deng Maria Bellizzi Dipali Rani Gupta Nur Uddin Mahmud Alfredo S.Urashima Sanjoy Kumar Paul Gary Peterson Yilin Zhou Xueping Zhou Md Tofazzal Islam Guo-Liang Wang 《Engineering》 SCIE EI 2021年第9期1326-1335,共10页
Wheat blast,caused by the fungus Magnaporthe oryzae Triticum(MoT)pathotype,is a devastating disease persistent in South America and Bangladesh.Since MoT generally fails to cause visual symptoms in wheat until the head... Wheat blast,caused by the fungus Magnaporthe oryzae Triticum(MoT)pathotype,is a devastating disease persistent in South America and Bangladesh.Since MoT generally fails to cause visual symptoms in wheat until the heading stage when the infection would have advanced,disease control by fungicide application solely based on the detection of visual symptoms is ineffective.To develop an accurate and sensitive method to detect MoT at the seedling and vegetative stages for disease control,we sequenced the genomes of two MoT isolates from Brazil and identified two DNA fragments,MoT-6098 and MoT-6099,that are present in the MoT genome but not in the genome of the rice-infecting Magnaporthe oryzae Oryzae(MoO)pathotype.Using polymerase chain reaction(PCR),we confirmed the specificity of the two markers in 53 MoT and MoO isolates from South America and Bangladesh.To test the efficiency of the two markers,we first established a loop-mediated isothermal amplification(LAMP)method to detect MoT at isothermal conditions,without the use of a PCR machine.Following this,we used the Cas12a protein and guide RNAs(gRNAs)to target the MoT-6098 and MoT-6099 sequences.The activated Cas12a showed indiscriminate single-stranded deoxyribonuclease(ssDNase)activity.We then combined targetdependent Cas12a ssDNase activation with recombinase polymerase amplification(RPA)and nucleic acid lateral flow immunoassay(NALFIA)to develop a method that accurately,sensitively,and cost-effectively detects MoT-specific DNA sequences in infected wheat plants.This novel technique can be easily adapted for the rapid detection of wheat blast and other important plant diseases in the field. 展开更多
关键词 Wheat blast Magnaporthe oryzae Triticum Cas12a Nucleic acid rapid lateral flow immunoassay Field detection
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Earthquake detection in the Jiangsu region, China using graphics-processing-unit-based Match & Locate and rapid earthquake association and location 被引量:3
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作者 Yafen Huang Shengzhong Zhang +3 位作者 Yuejun Lv Yanzhen Li Yuting Zhang Min Liu 《Earthquake Science》 2020年第1期23-33,共11页
Earthquake detection and location are essential in earthquake studies,which generally consists of two main classes:waveform-based and pick-based methods.To evaluate the ability of two different methods,a graphicsproce... Earthquake detection and location are essential in earthquake studies,which generally consists of two main classes:waveform-based and pick-based methods.To evaluate the ability of two different methods,a graphicsprocessing-unit-based Match&Locate(GPU-M&L)method and a rapid earthquake association and location(REAL)method are applied to continuous seismic data recorded by 24 digital seismic stations from Jiangsu Seismic Network during 2013 for comparison.GPU-M&L is one of waveform-based methods by waveform cross-correlations while REAL is one of pick-based method to associate arrivals of different seismic phases and locate events through counting the number of P and S picks and travel time residuals.Twenty-six templates are selected from the Jiangsu Seismic Network local catalog by using the GPU-M&L.The number of newly detected and located events is about 2.8 times more than those listed in the local catalog.We both utilize a deep-neural-network-based arrival-time picking method called PhaseNet and a shortterm/long-term average(STA/LTA)trigger algorithm for seismic phase detection and picking by applying the REAL.We then refine seismic locations using a least-squares location method(VELEST)and a high-precision relative location method(hypoDD).By applying STA/LTA and PhaseNet,1006 and 1893 events are associated and located,respectively.The newly detected events are mainly clustered and show steeply dipping fault planes.By analyzing the performance of these methods based on long-term continuous seismic data,the detected catalogs by the GPU-M&L and REAL show that the magnitudes of completeness are 1.4 and 0.8,respectively,which are smaller than 2.6 given by the local catalog.Although REAL provides improvement compared with GPU-M&L,REAL is highly dependent on phase detection and picking which is strongly affected by signal-noise ratio(SNR).Stations at southeast of the study region with low SNR may lead to few detections in the same area. 展开更多
关键词 earthquake detection rapid earthquake association and location graphics-processing-unit-based Match and Locate
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Rapid <i>In-Vitro</i>and <i>In-Vitro</i>Detection of <i>Chalara fraxinea</i>by Means of Mass Spectrometric Techniques 被引量:1
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作者 Thi Lam Huong Pham Irmtraut Zaspel +2 位作者 Michael Schuemann Heike Stephanowitz Eberhard Krause 《American Journal of Plant Sciences》 2013年第2期444-453,共10页
For the first time, mass spectrometric (MS) techniques were employed to rapidly detect the pathogen Chalara fraxinea in-vitro and directly in-vivo in tissues of diseased ash trees caused by C. fraxinea, using a range ... For the first time, mass spectrometric (MS) techniques were employed to rapidly detect the pathogen Chalara fraxinea in-vitro and directly in-vivo in tissues of diseased ash trees caused by C. fraxinea, using a range of characteristic novel secondary metabolites of C. fraxinea as chemical markers for the presence of the pathogen. We have found an evident correlation between the presence and amount of these-only for C. fraxinea characteristic and novel-secondary metabolites (named chalarafraxinines) and the degree of disease of respective infected ash seedlings. As demonstrated in this work, the MS based high-throughput-screening approach constitute an alternative to the time consuming and expensive micro biological isolation procedures for detection of the pathogen C. fraxinea and furthermore, can be used to rapidly test ash genotypes for resistance / susceptibility to C. fraxinea infection. 展开更多
关键词 Chalara fraxinea rapid In-Vitro In-Vitro detection MS TECHNIQUES MALDI LC-MS
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Detection of Environmental Toxins in Mixed Matrices of Tap Water, Soil, Food Waste, Serum and Milk Using Hememics Biosensor
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作者 Srivatsa Aithal Sujasha Gupta +5 位作者 Khanh Duong Ankit Kumar Nathan Ho Dongdong Liu John Warden David Huy Ho 《Journal of Sensor Technology》 2023年第4期59-68,共10页
Exposure to toxins can lead to a wide range of adverse health effects, including respiratory problems, neurological disorders, cancer, and reproductive issues. Toxins can come from various sources, such as industrial ... Exposure to toxins can lead to a wide range of adverse health effects, including respiratory problems, neurological disorders, cancer, and reproductive issues. Toxins can come from various sources, such as industrial waste, agricultural runoff, and household chemicals. Therefore, detecting and monitoring toxins in the environment is crucial for protecting human health and the environment. This study aimed to evaluate the performance of Hememics biosensor system in detecting environmental toxins such as Ricin and Staphylococcal enterotoxin B (SEB) in mixed matrixes. When Ricin and SEB are spiked into soil, chopped lettuce, tap water, milk and serum, the biosensor was able to detect these toxins, without sample processing, at a level of detection comparable to lab testing with high sensitivity and specificity. Furthermore, Hememics biosensor system is designed to be network-enabled, which means that results can be transmitted to relevant agencies for quick decisions. This feature is crucial in cases where quick action is needed to prevent further contamination or exposure to harmful toxins. 展开更多
关键词 Portable Biosensor Graphene Based Biochip HemChip™ rapid detection Field Use NETWORKING
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