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Cell/Tissue Mechanics optical tweezer,顯微鏡升級改造細(xì)胞力學(xué)光鑷

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  • 產(chǎn)品名稱:Cell/Tissue Mechanics optical tweezer,顯微鏡升級改造細(xì)胞力學(xué)光鑷
  • 產(chǎn)品型號:impetuxcomp
  • 產(chǎn)品展商:impetuxcomp
  • 產(chǎn)品文檔:無相關(guān)文檔
簡單介紹

Optical manipulation systems for quantitative cell and tissue mechanics 世聯(lián)博研公司代理的免校正多光阱細(xì)胞力學(xué)光鑷系統(tǒng)(多光阱細(xì)胞力學(xué)光鑷生物分子力學(xué)光鑷,細(xì)胞微流變學(xué)光鑷)可以在已有顯微鏡上升級配置起來,免校準(zhǔn)、使用簡潔方便、經(jīng)濟。 在活細(xì)胞中,免校準(zhǔn)力測量 多點中,活性微流變學(xué)測量 細(xì)胞力學(xué)研究的自動化例程 與

產(chǎn)品描述

世聯(lián)博研公司代理的免校正多光阱細(xì)胞力學(xué)光鑷系統(tǒng)(多光阱細(xì)胞力學(xué)光鑷生物分子力學(xué)光鑷,細(xì)胞微流變學(xué)光鑷)可以在已有顯微鏡上升級配置起來,免校準(zhǔn)、使用簡潔方便、經(jīng)濟。

impetux,Cygnium? G-422,LUNAM T-40i,DEIMUS T-10i細(xì)胞組織力學(xué)側(cè)量光鑷,細(xì)胞力學(xué)光鑷,多光阱細(xì)胞力學(xué)生物分子力學(xué)光鑷,單細(xì)胞力學(xué)光鑷,單分子力譜光鑷,馬達(dá)蛋白光鑷,微流變學(xué)光鑷

  • 在活細(xì)胞中,免校準(zhǔn)力測量
  • 多點中,活性微流變學(xué)測量
  • 細(xì)胞力學(xué)研究的自動化例程
  • 與相差、微分干涉或熒光顯微鏡兼容
  • 組織中力測量(厚0.5mm
  • 高效捕捉、低細(xì)胞損害
  • 樣品*大激光功率控制
  •  
  • 光鑷平臺由兩個單元組成:
  • 光操控模塊:用于顯微樣品的捕獲和運動
  • 力傳感器模塊:用于試驗中涉及的生物力的測量

可以在已有的顯微鏡上升級配置起來,簡潔方便經(jīng)濟

 

應(yīng)用范圍:

 

1. 單分子力譜

單分子力譜光鑷測量分析系統(tǒng)

 

?馬達(dá)蛋白

?DNA

?RNA

?蛋白-蛋白相互作用:配體受體;膜蛋白

2、馬達(dá)蛋白移動、運動

3、單細(xì)胞力學(xué)

細(xì)胞移動
細(xì)胞拉伸—膜彈性
細(xì)胞內(nèi)細(xì)胞器的操縱

4、微流變學(xué)

Key Bibliography

Here you will find useful material published related with our technology and products

Papers

  • Català, F. et al. “Extending calibration-free force measurements to optically-trapped rod-shaped samples“. Sci. Rep. 7, 42960; doi: 10.1038/srep42960 (2017).

Optical trapping has become an optimal choice for biological research at the microscale due to its noninvasiveperformance and accessibility for quantitative studies, especially on the forces involved inbiological processes. However, reliable force measurements depend on the calibration of the opticaltraps, which is different for each experiment and hence requires high control of the local variables,especially of the trapped object geometry. Many biological samples have an elongated, rod-likeshape, such as chromosomes, intracellular organelles (e.g., peroxisomes), membrane tubules, certainmicroalgae, and a wide variety of bacteria and parasites. This type of samples often requires severaloptical traps to stabilize and orient them in the correct spatial direction, making it more difficult todetermine the total force applied. Here, we manipulate glass microcylinders with holographic opticaltweezers and show the accurate measurement of drag forces by calibration-free direct detection ofbeam momentum.

  • R. Bola, F. Català. M. Montes-Usategui, E. Martín-Badosa. Optical tweezers for force measurements and rheological studies on biological samples”.15th workshop on Information Optics (WIO), 2016.

Measuring forces inside living cells is still a challenge due the characteristics of the trapped organelles (non-spherical, unknown size and index of refraction) and the cell cytoplasm surrounding them heterogeneous and dynamic, non-purely viscous). Here, we show how two very recent methods overcome these limitations: on the one hand, forces can be measured in such environment by the direct detection of changes in the light momentum; on the other hand, an active-passive calibration technique provides both the stiffness of the optical trap as well as the local viscoelastic properties of the cell cytoplasm.

  • Martín-Badosa, F. Català, J. Mas, M. Montes-Usategui, A. Farré, F. Marsà. “Force measurement in the manipulation of complex samples with holographic optical tweezers”15th workshop on Information Optics (WIO), 2016.
  • Derek Craig, Alison McDonald, Michael Mazilu, Helen Rendall, Frank Gunn-Moore, and Kishan Dholakia. “ Enhanced Optical Manipulation of Cells Using Antireflection Coated Microparticles”.ACS Photonics, 2 (10), pp 1403–1409, (2015).

    In molecular studies, an optically trapped bead may be functionalized to attach to a specific molecule, whereas in cell studies, direct manipulation with the optical field is usually employed. Using this approach, several methods may be used to measure forces with an optical trap. However, each has its limitations and requires an accurate knowledge of the sample parameters.6,7 In particular, force measurements can be challenging when working with nonspherical particles or in environments with an inhomogeneous viscosity, such as inside the cell. Recent developments in the field are moving toward obtaining direct force measurements by detecting light momentum changes. For this approach, the calibration factor only comes from the detection instrumentation and negates the requirement to recalibrate for changes in experimental conditions”.

  • Xing Ma, Anita Jannasch, Urban-Raphael Albrecht, Kersten Hahn, Albert Miguel-López, Erik Sch?ffer, and Samuel Sánchez. “Enzyme-Powered Hollow Mesoporous Janus Nanomotors”. Nano Lett., 15 (10), pp 7043–7050, (2015).

    “Using optical tweezers, we directly measured a holding force of 64 ± 16 fN, which was necessary to counteract the effective self-propulsion force generated by a single nanomotor. The successful demonstration of biocompatible enzyme-powered active nanomotors using biologically benign fuels has a great potential for future biomedical applications.”

  • Michael A. Taylor, Muhammad Waleed, Alexander B. Stilgoe, Halina Rubinsztein-Dunlop and Warwick P. Bowen. “Enhanced optical trapping via structured scattering“. Nature Photonics 9,669–673 (2015)
  • Gregor Thalhammer, Lisa Obmascher, and Monika Ritsch-Marte, “Direct measurement of axial optical forces“.Optics Express, Vol. 23, Issue 5, pp. 6112-6129 (2015)
  • Y. Jun, S.K. Tripathy, B.R.J. Narayanareddy, M. K. Mattson-Hoss, S.P. Gross, “Calibration of Optical Tweezers for In Vivo Force Measurements: How do Different Approaches Compare?”. Biophysical Journal, V 107, 1474-1484 (2014).

    Here, the authors present a comparison between two different methods for measuring forces inside living cells and provide measurements of the stall force of kinesin in vivo using the momentum-based approach. More information at: http://bioweb.bio.uci.edu/sgross/publications.html

  • A. Farré, E. Martín-Badosa, and M. Montes-Usategui, “The measurement of light momentum shines the path towards the cell”, Opt. Pur Apl. 47, 239-248 (2014).
  • A. Farré, F. Marsà, and M. Montes-Usategui, “A force measurement instrument for optical tweezers based on the detection of light momentum changes”, Proc. SPIE 9164, 916412 (2014).
  • J. Mas, A. Farré, J. Sancho-Parramon, E. Martín-Badosa, and M. Montes-Usategui, “Force measurements with optical tweezers inside living cells”,  Proc. SPIE 9164, 91640U (2014).
  • F. Català, F. Marsà, A. Farré, M. Montes-Usategui, and E. Martín-Badosa, “Momentum measurements with holographic optical tweezers for exploring force detection capabilities on irregular samples”, Proc. SPIE 9164, 91640A (2014).
  • A. Farré, F. Marsà, and M. Montes-Usategui, “Optimized back-focal-plane interferometry directly measures forces of optically trapped particles” Opt. Express 20, 12270-12291 (2012).

    This manuscript shows the relation between the determination of momentum measurements and back-focal-plane interferometry, and details how to obtain the force response of the sensor both from first principles and from its connection with trap stiffness calibration.

  • A. Farré and M. Montes-Usategui, “A force detection technique for single-beam optical traps based on direct measurement of light momentum changes” Opt. Express 18, 11955-11968 (2010).

 In this work, the authors show the feasibility of combining optical tweezers (single-beam gradient traps) with the determination of forces using the measurement of the light momentum change.



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