上转换发光成像技术与靶向成像应用

上转换发光是指稀土离子吸收两个或两个以上低能光子(近红外光)而辐射一个高能光子(可见光)的发光现象。与传统紫外激发相比,上转换发光由于采用近红外光激发而具有高的组织穿透深度、弱的生物样品损伤且无生物样品自发荧光,这些优点表明上转换发光在生物成像方面具有广阔的应用前景。文章介绍了基于稀土上转换发光过程的显微成像技术和活体成像技术,及其在肿瘤靶向成像领域的应用。     

多光子显微成像技术在脑部疾病研究中的应用

由于多光子显微技术具有高时空分辨率、低损伤性、可对活体长时间成像等特点,近年来已被广泛应用于生物医学等领域,并且在多种疾病诊断中展现出巨大的应用潜力.尤其是在脑部疾病的研究中,利用多光子成像技术可实现对复杂神经网络的研究,包括对脑部神经细胞、血管、肿瘤等进行实时成像并研究各自之间的相互作用,能进一步揭示脑疾病的发病机制并指导检测治疗方法的开发.本文简要介绍了多光子成像技术的基本原理及特点,总结了其在阿尔茨海默病、脑中风、脑肿瘤等多种脑部疾病中的应用,详细阐述了近年来利用多光子成像技术在脑部疾病研究中所获得的成果,并对多光子成像技术的发展前景进行了展望,预期其在脑部疾病的研究中将发挥更大的作用.     

生物科学研究中的激光多光子显微技术

本文综述了生物科学中近红外（NIR）多光子激光扫描显微技术的进展,其中包括：多光子显微特点,激光光源,荧光寿命的测量,多光子多色实时杂化荧光（FISH）,非人侵性活体光学解剖,植物学中的多光子显微技术,细胞的多光子显微损伤、皮米非入侵和非接触性外科手术等。     

双光子激发荧光各向异性度的成像

荧光各向异性度 (fluorescence anisotropy) 测量可以获得荧光分子的转动速度信息,进而了解分子质量、结构、以及与周边环境的相互作用情况 . 围绕一台双光子激发扫描荧光成像系统,通过改变外光路和图像记录与处理程序,从而实现了双光子激发荧光各向异性度成像,并针对一些典型样品和体系,展示了该方法的应用 . 实验中观察了 FITC 荧光分子、 FITC 结合的 CD44 抗体分子及与肿瘤细胞表面受体结合的 FITC-CD44 抗体分子 . 测量结果表明,不同分子质量、不同微观环境状态下的荧光分子,其各向异性度大小不同,在各向异性度图中能够被明显区分 . 荧光各向异性度成像能够定量测量样品微区的各向异性度值,并以二维图像的形式直观表达,是各向异性度测量与成像技术的良好结合 .     

活细胞内5-羟色胺可见荧光的多光子激发成像

应用多光子激发激光扫描显微镜对5-羟色胺（5-hydroxytryptamine, 5-HT）孵育的大鼠粘膜型肥大细胞进行自发荧光成像,首次观察到了活细胞内5-HT相关的可见荧光,并对其产生机理进行了初步探讨.实现了对活细胞内5-HT空间分布的高分辨成像,为研究活组织或细胞内5-HT的空间分布和含量与细胞功能状态的关系提供了新的实验方法.     

多光子显微镜在研究阿尔茨海默病中的应用

多光子显微镜采用近红外线激发荧光成像,能直接观察AD老年斑的自然病理进展,并且在鼠模型中进行抗老年斑治疗的疗效评估.其高分辨率的特点,可用于监测蛋白与蛋白之间、蛋白构象改变和蛋白水解而产生的荧光共振能量转移(FRET)改变.     

多光子激发技术及其在生命科学中的应用

多光子激发技术是20世纪90年代初发展起来的新技术,其研究和应用前景十分广阔。本文对多光子激发的原理,优缺点以及近年来它的应用领域作了简介。     

综述与专论: 肝脏免疫的活体显微光学成像研究进展

光学分子成像技术是在活体复杂的组织区域环境内细胞形态、运动与功能研究的最佳手段之一,极大地推进了免疫学的发展．肝脏是机体新陈代谢和解毒的重要器官,也被视为一个免疫器官．解析肝脏免疫基本特性和功能,对防治肝脏疾病以及全身性相关疾病具有重要意义．活体可视化研究肝脏区域生理或者病理状态下免疫应答,提供关键事件的多细胞参与及其彼此交互的时空动态信息,能极大地丰富对肝脏独特免疫反应的认知．本文将重点阐述目前活体肝脏成像的技术与方法以及光学显微成像技术,例如多光子激发显微成像与转盘共聚焦成像在肝脏免疫中的应用,并展望活体肝脏成像今后的发展方向和面临的机遇与挑战．     

双光子显微成像系统群延迟色散的测量和补偿

为了对双光子显微成像系统的群延迟色散进行校正,提高双光子激发效率的目的,采用自相关仪测量的方法在自行搭建的双光子系统光路的四个位置测量飞秒激光的脉冲展宽情况,测量样品位置5个波长下最优的群延迟色散补偿值,由此拟合得到自搭建双光子系统的全波段群延迟色散补偿曲线。实验结果表明在应用此群延迟色散补偿曲线后样品位置的脉冲宽度平均减小95 fs,在两个典型激发波长(750 nm和900 nm)生物样品的荧光强度分别提高了42.7%和76.8%。结论为双光子激发效率与飞秒激光的脉冲宽度成线性反比关系。     

可用于双色双光子显微成像的新的荧光蛋白对

双色双光子激光扫描显微技术可以用来研究生物组织内两种不同蛋白质的表达、定位和示踪．由于大多数双光子显微镜一次只能提供一种波长的激发光,双色同时成像较难实现．mAmetrine和mKate2作为新发现的荧光蛋白对可以用于双光子双色同时成像,这得益于它们各自的优势：mAmetrine的斯托克斯位移和mKate2的高亮度．在765nm的波长激发时,它们的双光子吸收效率都很高．mAmetrine和mKate2能够很好地用于双色双光子活细胞成像实验．     

Simultaneous two-photon calcium imaging at different depths with spatiotemporal multiplexing

In vivo two-photon calcium imaging would benefit from the use of multiple excitation beams to increase scanning speed, signal-to-noise ratio and field of view or to image different axial planes simultaneously. Using spatiotemporal multiplexing we circumvented light-scattering ambiguity inherent to deep-tissue multifocal two-photon microscopy. We demonstrate calcium imaging at multiple axial planes in the intact mouse brain to monitor network activity of ensembles of cortical neurons in three spatial dimensions.     

Laser tweezers and multiphoton microscopes in life sciences

Near infrared (NIR) laser microscopy enables optical micromanipulation, piconewton force determination, and sensitive fluorescence studies by laser tweezers. Otherwise, fluorescence images with high spatial and temporal resolution of living cells and tissues can be obtained via non-resonant fluorophore excitation with multiphoton NIR laser scanning microscopes. Furthermore, NIR femtosecond laser pulses at TW/cm2 intensities can be used to realize non-invasive contact-free surgery of nanometer-sized structures within living cells and tissues. Applications of these novel versatile NIR laser-based tools for the determination of motility forces, coenzyme and chlorophyll imaging, three-dimensional multigene detection, non-invasive optical sectioning of tissues ("optical biopsy"), functional protein imaging, and nanosurgery of chromosomes are described.     

Live cell imaging by multifocal multiphoton microscopy

Multifocal multiphoton microscopy (MMM) permits parallel multiphoton excitation by scanning an array of high numerical aperture foci across a plane in the sample. MMM is particularly suitable for live cell investigations since it combines advantages of standard multiphoton microscopy such as optical sectioning and suppression of out-of-focus phototoxicity with high recording speeds. Here we describe several applications of MMM to live cell imaging using the neuroendocrine cell line PC12 and bovine chromaffin cells. Stainings were performed with the acidophilic dye acridine orange and the lipophilic dyes FM1-43 and Fast DiA as well as by transfection of the cells with GFP. In both bovine chromaffin and PC12 cells structural elements of nuclear chromatin and the 3-D distribution of acidic organelles inside the cells were visualized. In PC12 cells differentiated by nerve growth factor examples of neurites were monitored. Stainings of membranes were used to reconstruct the morphology of cells and neurites in three dimensions by volume-rendering and by isosurface plots. 3-D reconstructions were composed from stacks of about 50 images each with a diameter of 30-100 microm that were acquired within a few seconds. We conclude that MMM proves to be a technically simple and very effective method for fast 3-D live cell imaging at high resolution.     

东海剧毒卡尔藻的形态特征及其系统进化分析

利用光学显微镜、荧光显微镜、扫描电镜及分子生物学等方法, 对分布于我国东海海域的剧毒卡尔藻（Karlodinium veneficum）藻株（LAMB090611）的形态特征和显微结构进行了描述, 并探讨了其分子系统进化关系。该藻株细胞长11.1-18.7 μm, 平均值为（14.2±1.8） μm, 宽8.2-14.7 μm, 平均值为（10.8±1.5） μm。细胞形态结构特征为： 上下锥体积基本相同; 顶沟短而直; 腹孔明显; 纵沟延伸至上锥; 横沟错位距离约占细胞总长的28%-38%; 含有2或4个不规则形态的叶绿体; 细胞核位于中部或下锥。此藻种的暴发可引发有害赤潮（harmful algal bloom）。当前加强有害赤潮的预防和监测工作是减少危害的有效途径, 而对引发赤潮原因种的准确识别和鉴定则是基础和关键。     

Characteristics of a novel deep red/infrared fluorescent cell-permeant DNA probe, DRAQ5, in intact human cells analyzed by flow cytometry, confocal and multiphoton microscopy

BACKGROUND: The multiparameter fluorometric analysis of intact and fixed cells often requires the use of a nuclear DNA discrimination signal with spectral separation from visible range fluorochromes. We have developed a novel deep red fluorescing bisalkylaminoanthraquinone, DRAQ5 (Ex(lambdamax) 646 nm; Em(lambdamax) 681 nm; Em(lambdarange) 665->800 nm), with high affinity for DNA and a high capacity to enter living cells. We describe here the spectral characteristics and applications of this synthetic compound, particularly in relation to cytometric analysis of the cell cycle. METHODS: Cultured human tumor cells were examined for the ability to nuclear locate DRAQ5 using single and multiphoton laser scanning microscopy (LSM) and multiparameter flow cytometry. RESULTS: Multiparameter flow cytometry shows that the dye can rapidly report the cellular DNA content of live and fixed cells at a resolution level adequate for cell cycle analysis and the cycle-specific expression of cellular proteins (e.g., cyclin B1). The preferential excitation of DRAQ5 by laser red lines (633/647 nm) was found to offer a means of fluorescence signal discrimination by selective excitation, with greatly reduced emission overlap with UV-excitable and visible range fluophors as compared with propidium iodide. LSM reveals nuclear architecture and clearly defines chromosomal elements in live cells. DRAQ5 was found to permit multiphoton imaging of nuclei using a 1,047-nm emitting mode-locked YLF laser. The unusual spectral properties of DRAQ5 also permit live cell DNA analysis using conventional 488 nm excitation and the single-photon imaging of nuclear fluorescence using laser excitation between 488 nm and low infrared (IR; 780 nm) wavelengths. Single and multiphoton microscopy studies revealed the ability of DRAQ5 to report three-dimensional nuclear structure and location in live cells expressing endoplasmic reticulum targeted-GFP, MitoTracker-stained mitochondria, or a vital cell probe for free zinc (Zinquin). CONCLUSION: The fluorescence excitation and emission characteristics of DRAQ5 in living and fixed cells permit the incorporation of the measurement of cellular DNA content into a variety of multiparameter cytometric analyses.     

Low‐photobleaching line‐scanning confocal microscopy using dual inclined beams

Confocal microscopy is an indispensable tool for biological imaging due to its high resolution and optical sectioning capability. However, its slow imaging speed and severe photobleaching have largely prevented further applications. Here, we present dual inclined beam line‐scanning (LS) confocal microscopy. The reduced excitation intensity of our imaging method enabled a 2‐fold longer observation time of fluorescence compared to traditional LS microscopy while maintaining a good sectioning capability and single‐molecule sensitivity. We characterized the performance of our method and applied it to subcellular imaging and three‐dimensional single‐molecule RNA imaging in mammalian cells.      

Tracking metastatic tumor cell extravasation with quantum dot nanocrystals and fluorescence emission-scanning microscopy

Metastasis is an impediment to the development of effective cancer therapies. Our understanding of metastasis is limited by our inability to follow this process in vivo. Fluorescence microscopy offers the potential to follow cells at high resolution in living animals. Semiconductor nanocrystals, quantum dots (QDs), offer considerable advantages over organic fluorophores for this purpose. We used QDs and emission spectrum scanning multiphoton microscopy to develop a means to study extravasation in vivo. Although QD labeling shows no deleterious effects on cultured cells, concern over their potential toxicity in vivo has caused resistance toward their application to such studies. To test if effects of QD labeling emerge in vivo, tumor cells labeled with QDs were intravenously injected into mice and followed as they extravasated into lung tissue. The behavior of QD-labeled tumor cells in vivo was indistinguishable from that of unlabeled cells. QDs and spectral imaging allowed the simultaneous identification of five different populations of cells using multiphoton laser excitation. Besides establishing the safety of QDs for in vivo studies, our approach permits the study of multicellular interactions in vivo.     

Optical microscopy in photosynthesis

Emerging as well as the most frequently used optical microscopy techniques are reviewed and image contrast generation methods in a microscope are presented, focusing on the nonlinear contrasts such as harmonic generation and multiphoton excitation fluorescence. Nonlinear microscopy presents numerous advantages over linear microscopy techniques including improved deep tissue imaging, optical sectioning, and imaging of live unstained samples. Nonetheless, with the exception of multiphoton excitation fluorescence, nonlinear microscopy is in its infancy, lacking protocols, users and applications; hence, this review focuses on the potential of nonlinear microscopy for studying photosynthetic organisms. Examples of nonlinear microscopic imaging are presented including isolated light-harvesting antenna complexes from higher plants, starch granules, chloroplasts, unicellular alga Chlamydomonas reinhardtii, and cyanobacteria Leptolyngbya sp. and Anabaena sp. While focusing on nonlinear microscopy techniques, second and third harmonic generation and multiphoton excitation fluorescence microscopy, other emerging nonlinear imaging modalities are described and several linear optical microscopy techniques are reviewed in order to clearly describe their capabilities and to highlight the advantages of nonlinear microscopy.     

Multiphoton excitation provides optical sections from deeper within scattering specimens than confocal imaging.

Multiphoton excitation fluorescence imaging generates an optical section of sample by restricting fluorophore excitation to the plane of focus. High photon densities, achieved only in the focal volume of the objective, are sufficient to excite the fluorescent probe molecules by density-dependent, multiphoton excitation processes. We present comparisons of confocal with multiphoton excitation imaging of identical optical sections within a sample. These side-by-side comparisons of imaging modes demonstrate a significant advantage of multiphoton imaging; data can be obtained from deeper within biological specimens. Observations on a variety of biological samples showed that in all cases there was at least a twofold improvement in the imaging penetration depth obtained with multiphoton excitation relative to confocal imaging. The more pronounced degradation in image contrast deep within a confocally imaged sample is primarily due to scattered emission photons, which reduce the signal and increase the local background as measurements of point spread functions indicated that resolution does not significantly change with increasing depth for either mode of microscopy. Multiphoton imaging does not suffer from degradation of signal-to-background to nearly the same extent as confocal imaging because this method is insensitive to scatter of the emitted signal. Direct detection of emitted photons using an external photodetector mounted close to the objective (possible only in a multiphoton imaging system) improves system sensitivity and the utilization of scattered emission photons for imaging. We demonstrate that this technique provides yet further improvements in the capability of multiphoton excitation imaging to produce good quality images from deeper within tissue relative to confocal imaging.