Leica TCS SP8 STED 3X超高分辨率激光共聚焦顯微鏡
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Leica TCS SP8 STED 3X超高分辨率激光共聚焦顯微鏡
儀器簡(jiǎn)介:
STED 3X 顯微技術(shù)*集成在TCS SP8平臺(tái)中。使用TCS SP8 STED 3X,可以獲得共聚焦的精髓。的光學(xué)元件與配備有 HyD™的多光譜檢測(cè)系統(tǒng)以及徠卡白激光相結(jié)合,不但可以增強(qiáng)靈敏度和對(duì)比度,還可同時(shí)降低激光照射功率。因此,即使是染色不佳的樣品,也可以得到真實(shí)的超高分辨率光學(xué)切片圖像。共振掃描技術(shù)輔以門(mén)控STED,幫助您獲得*的超高分辨率活細(xì)胞圖像。12kHZ 高速掃描鏡能夠在zui快的速度下,以512×16格式記錄多達(dá)420fps超高分辨率圖像。同時(shí)也可以利用STED-FCS(STED-熒光相關(guān)光譜)進(jìn)行單分子檢測(cè)(SMD)。徠卡創(chuàng)新技術(shù)相輔相成,受益無(wú)限。
三維的STED-所有維度的超高分辨率,依靠TCS SP8 STED 3X,您可以根據(jù)您的需要自由設(shè)計(jì)PSF,從而選擇XY和Z方向上的*分辨率。
多色成像-在整個(gè)光譜范圍上的超高分辨率 TCS SP8 STED 3X可提供多條STED激光線。更多的熒光染料可以被用于STED成像。
活細(xì)胞成像-高速超高分辨率成像,門(mén)控STED提高了染料的光穩(wěn)定性,并且提高了系統(tǒng)的活細(xì)胞性能。
應(yīng)用范圍:
主要用于組織切片、活細(xì)胞的熒光標(biāo)記、三維圖像重建分析研究;細(xì)胞生物物質(zhì)、離子的定性、定量、定時(shí)和定位分布檢測(cè)等,可以在同一張樣品上同時(shí)進(jìn)行多重?zé)晒鈽?biāo)記觀察。對(duì)活細(xì)胞或組織切片進(jìn)行連續(xù)掃描,可獲得精細(xì)的細(xì)胞骨架、染色體、細(xì)胞器和細(xì)胞膜系統(tǒng)的三維圖像。與普通熒光顯微鏡相比,具有更高對(duì)比度、解析度和高靈敏度。
技術(shù)規(guī)格:
- 在x、y和z中靈活可調(diào)的直接超分辨率,展示了zui精細(xì)的細(xì)節(jié)信息。
- 多條STED光線實(shí)現(xiàn)了可見(jiàn)光的全光譜超高分辨率成像。
- 門(mén)控檢測(cè)提高了分辨率以及活細(xì)胞性能。
- STED白色物鏡為全光譜范圍提供*色差校正。
- 自動(dòng)光束校準(zhǔn)保證系統(tǒng)的穩(wěn)定性和結(jié)果的可靠性。
- 基于TCS SP8的模塊化設(shè)計(jì)可隨時(shí)升級(jí)。
- 智能STED向?qū)Э芍庇^地控制實(shí)驗(yàn)。
- 惠更斯反卷積可以從原始數(shù)據(jù)中獲取更多信息。
STED Key Publications
First publication on STED technology:
Hell, S. W. & Wichmann, J. Breaking the diffraction resolution limit by stimulated emission: stimulated-emission-depletion fluorescence microscopy. Optics letters 19, 780-782, (1994).http://www.ncbi.nlm.nih.gov/pubmed/19844443
First biological image:
Klar, T. A., Jakobs, S., Dyba, M., Egner, A. & Hell, S. W. Fluorescence microscopy with diffraction resolution barrier broken by stimulated emission. Proceedings of the National Academy of Sciences of the United States of America 97, 8206-8210, (2000). http://www.ncbi.nlm.nih.gov/pubmed/10899992
STED with genetically encoded marker: GFP
Willig, K. I. et al. Nanoscale resolution in GFP-based microscopy. Nature methods 3, 721-723, (2006).http://www.ncbi.nlm.nih.gov/pubmed/16896340
STED with continuous wave laser beams:
Willig, K. I., Harke, B., Medda, R. & Hell, S. W. STED microscopy with continuous wave beams. Nature methods 4, 915-918, (2007). http://www.ncbi.nlm.nih.gov/pubmed/17952088
Two-color STED with two STED lines
Donnert, G. et al. Two-color far-field fluorescence nanoscopy. Biophysical journal 92, L67-69, (2007).http://www.ncbi.nlm.nih.gov/pubmed/17307826
Iso-STED and two-color STED with one STED line
Schmidt, R. et al. Spherical nanosized focal spot unravels the interior of cells. Nature methods 5, 539-544, (2008).http://www.ncbi.nlm.nih.gov/pubmed/18488034
STED-FCS application
Eggeling, C. et al. Direct observation of the nanoscale dynamics of membrane lipids in a living cell. Nature 457, 1159-1162, (2009). http://www.ncbi.nlm.nih.gov/pubmed/19098897
Gated STED
Vicidomini, G. et al. Sharper low-power STED nanoscopy by time gating. Nature methods 8, 571-573, (2011).http://www.ncbi.nlm.nih.gov/pubmed/21642963
Selected Publications with Leica STED instrument
2016
Qiu, Z. et al. Translation Microscopy (TRAM) for super-resolution imaging. Scientific reports 6, 19993, (2016).http://www.ncbi.nlm.nih.gov/pubmed/26822455
Ruge, C. A. et al. Disintegration of nano-embedded microparticles after deposition on mucus: A mechanistic study. Colloids and surfaces. B, Biointerfaces 139, 219-227, (2016). http://www.ncbi.nlm.nih.gov/pubmed/26720142
Scheuring, D. et al. Actin-dependent vacuolar occupancy of the cell determines auxin-induced growth repression. Proceedings of the National Academy of Sciences of the United States of America 113, 452-457, (2016).http://www.ncbi.nlm.nih.gov/pubmed/26715743
Torreno-Pina, J. A. et al. The actin cytoskeleton modulates the activation of iNKT cells by segregating CD1d nanoclusters on antigen-presenting cells. Proceedings of the National Academy of Sciences of the United States of America 113, E772-781, (2016). http://www.ncbi.nlm.nih.gov/pubmed/26798067