Label-Free Chemical Imaging for Biological Applications
用于生物应用的无标记化学成像
基本信息
- 批准号:8352315
- 负责人:
- 金额:$ 240万
- 依托单位:
- 依托单位国家:美国
- 项目类别:
- 财政年份:2012
- 资助国家:美国
- 起止时间:2012-09-30 至 2017-06-30
- 项目状态:已结题
- 来源:
- 关键词:Action PotentialsAnimal ModelAreaBiochemicalBiochemistryBiologicalBiologyBiomedical ResearchCaenorhabditis elegansCell membraneCellsChemicalsCholesterolDetectionDrug Delivery SystemsDrug KineticsFaceFatty acid glycerol estersFluorescenceFrequenciesGenesGeneticGenetic ScreeningGenomeGoalsImageImaging TechniquesLabelLifeLightLipidsMechanicsMembrane LipidsMembrane PotentialsMetabolic DiseasesMicroscopyMonitorNeurobiologyNeuronsNeurosciencesNeurotransmittersObesityOptical MethodsOpticsOrganismPerformancePharmaceutical PreparationsProblem SolvingRNA InterferenceRadiationResearchResolutionSamplingSchemeScreening procedureSecond Messenger SystemsSensitivity and SpecificitySignal TransductionSpecificityStagingTechniquesTimeUnsaturated Fatsabstractingcancer diagnosischemical bondcombatelectric fieldfluorescence imaginggene discoveryimaging modalityinfancyinnovationinterestlight microscopylipid metabolismmulti-photonnoveloptical imagingpublic health relevancequantumsecond messengersmall moleculevoltage
项目摘要
DESCRIPTION (Provided by the applicant)
Abstract: Fluorescence is the most popular optical contrast for studying live cells. However, fluorescence imaging faces fundamental limitations for probing a vast number of small bio-molecules such as metabolites (e.g., ATP), second messengers, neurotransmitters and drugs. Most of these molecules are intrinsically non-fluorescent. Moreover, labeling them is not feasible, because their biochemical activities would be strongly altered by bulky probes. Thus, how to image these species inside live cells represents a grand challenge. Novel imaging techniques that accomplish this goal would undoubtedly open up new avenues, transforming our ability to monitor biochemistry in living systems in real time. We propose to solve this problem using an emerging multi-photon optical imaging method: stimulated radiation microscopy. By harnessing the power of stimulated Raman scattering (SRS), which serves as a quantum mechanical mechanism for light amplification, chemical contrast from the vibrating chemical bonds in the sample can be generated with high resolution in 3D without adding any external labels. While SRS microscopy is transforming label-free chemical imaging, the technique is still in its infancy. Particularly, both the detection sensitivity and specificity, th key performance criteria, are not high enough for SRS to be truly revolutionary. Many interesting molecules are still beyond detection. We propose to bring the technique to the stage where it can be widely applied to most small bio-molecules. Our plans are: (1) to couple SRS excitation with photo-thermal dark field imaging, a background-free detection scheme estimated to be ~100 times more sensitive; and (2) to use a broadband wavelength multiplex approach to significantly enhance the detection specificity, which should be able to distinguish more closely related chemical species. We are applying stimulated radiation to tackle two compelling problems in lipid biology and neurobiology: (1) Genetic screening for fat-regulating genes by chemical imaging. In order to identify new genes regulating fat metabolism, we will combine SRS lipid imaging with RNA interference screening. We have recently demonstrated such a novel combination of imaging and genetics with C. elegans. The proposed sensitivity boost would expand the screening to the genome scale, and the specificity enhancement should allow us to probe unsaturated lipid and cholesterol. (2) Optical monitoring of membrane potentials. Despite of many efforts, there is no satisfactory optical method to monitor voltage signal in neurons. The intense electric field across the plasma membranes during action potentials should shift the vibrational frequency of membrane lipids, and we plan to employ this vibrational electrochromism as a label-free contrast mechanism for voltage imaging. The proposed technical innovation has the potential to greatly advance light microscopy, lipid biology, genetic screening and neuroscience, and the applications will take bio-imaging into new areas of biomedicine that have been previously uncharted.
Public Health Relevance: The unprecedented ability to visualize small molecules such as metabolites and drugs in living cells and organisms without any labels will revolutionize many areas of biomedical research, particularly lipid biology, pharmacokinetics and cancer diagnosis. The proposed genetic screening research would discover genes that regulate fat metabolism and distribution on the multicellular organism models. These newly identified genes could become potential drug targets for combating obesity and related metabolic disorders.
描述(由申请人提供)
项目成果
期刊论文数量(7)
专著数量(0)
科研奖励数量(0)
会议论文数量(0)
专利数量(2)
Live-cell imaging of alkyne-tagged small biomolecules by stimulated Raman scattering.
- DOI:10.1038/nmeth.2878
- 发表时间:2014-04
- 期刊:
- 影响因子:48
- 作者:Wei, Lu;Hu, Fanghao;Shen, Yihui;Chen, Zhixing;Yu, Yong;Lin, Chih-Chun;Wang, Meng C.;Min, Wei
- 通讯作者:Min, Wei
Live-cell quantitative imaging of proteome degradation by stimulated Raman scattering.
- DOI:10.1002/anie.201310725
- 发表时间:2014-05-26
- 期刊:
- 影响因子:16.6
- 作者:Shen, Yihui;Xu, Fang;Wei, Lu;Hu, Fanghao;Min, Wei
- 通讯作者:Min, Wei
Live-cell vibrational imaging of choline metabolites by stimulated Raman scattering coupled with isotope-based metabolic labeling.
- DOI:10.1039/c3an02281a
- 发表时间:2014-05-21
- 期刊:
- 影响因子:0
- 作者:Hu F;Wei L;Zheng C;Shen Y;Min W
- 通讯作者:Min W
Imaging complex protein metabolism in live organisms by stimulated Raman scattering microscopy with isotope labeling.
- DOI:10.1021/cb500787b
- 发表时间:2015-03-20
- 期刊:
- 影响因子:4
- 作者:Wei L;Shen Y;Xu F;Hu F;Harrington JK;Targoff KL;Min W
- 通讯作者:Min W
Multicolor live-cell chemical imaging by isotopically edited alkyne vibrational palette.
- DOI:10.1021/ja502706q
- 发表时间:2014-06-04
- 期刊:
- 影响因子:15
- 作者:Chen, Zhixing;Paley, Daniel W.;Wei, Lu;Weisman, Andrew L.;Friesner, Richard A.;Nuckolls, Colin;Min, Wei
- 通讯作者:Min, Wei
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Wei Min其他文献
Wei Min的其他文献
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{{ truncateString('Wei Min', 18)}}的其他基金
Super-multiplex optical imaging: development of novel spectroscopy and probes to illuminate complex biomedicine
超级多重光学成像:开发新型光谱学和探针来阐明复杂的生物医学
- 批准号:
10622905 - 财政年份:2023
- 资助金额:
$ 240万 - 项目类别:
High-resolution volumetric imaging of metabolic activity in tissues and its application to tumor metabolism
组织代谢活动的高分辨率体积成像及其在肿瘤代谢中的应用
- 批准号:
10376225 - 财政年份:2020
- 资助金额:
$ 240万 - 项目类别:
High-resolution volumetric imaging of metabolic activity in tissues and its application to tumor metabolism
组织代谢活动的高分辨率体积成像及其在肿瘤代谢中的应用
- 批准号:
10551256 - 财政年份:2020
- 资助金额:
$ 240万 - 项目类别:
High-resolution volumetric imaging of metabolic activity in tissues and its application to tumor metabolism
组织代谢活动的高分辨率体积成像及其在肿瘤代谢中的应用
- 批准号:
10117249 - 财政年份:2020
- 资助金额:
$ 240万 - 项目类别:
Ultrahigh-resolution and single-molecule stimulated Raman scattering (SRS) microscopy
超高分辨率单分子受激拉曼散射 (SRS) 显微镜
- 批准号:
9899269 - 财政年份:2019
- 资助金额:
$ 240万 - 项目类别:
Ultrahigh-resolution and single-molecule stimulated Raman scattering (SRS) microscopy
超高分辨率单分子受激拉曼散射 (SRS) 显微镜
- 批准号:
10377375 - 财政年份:2019
- 资助金额:
$ 240万 - 项目类别:
Super-multiplex vibrational imaging in living cells
活细胞中的超多重振动成像
- 批准号:
10163876 - 财政年份:2018
- 资助金额:
$ 240万 - 项目类别:
Super-multiplex vibrational imaging in living cells
活细胞中的超多重振动成像
- 批准号:
9921414 - 财政年份:2018
- 资助金额:
$ 240万 - 项目类别:
Optical imaging of small bio-molecules in living cells and tissues by nonlinear Raman microscopy coupled with vibrational tags
通过非线性拉曼显微镜结合振动标签对活细胞和组织中的小生物分子进行光学成像
- 批准号:
9298651 - 财政年份:2015
- 资助金额:
$ 240万 - 项目类别:
Stimulated emission reduced fluorescence (SERF) for breaking and extending the fundamental imaging-depth of two photon microscopy
受激发射减少荧光 (SERF) 用于打破和扩展双光子显微镜的基本成像深度
- 批准号:
9025791 - 财政年份:2015
- 资助金额:
$ 240万 - 项目类别:
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