快速global mapping(非扫描式)
百万像素拉曼光谱,成像时间仅几分钟
斯托克斯和反斯托克斯
高光谱分辨率和空间分辨率
Photon etc公司RIMA拉曼成像技术是新一代快速、高精度、面扫描激光拉曼技术,它将共聚焦显微技术与激光拉曼光谱技术**结合,与传统的点成像拉曼系统不同,采用面成像技术,将激光扩束后,用特殊的光学元件将扩束后的高斯分布的激光整形成均匀分布的平顶激光,照射在样品上,滤除反射的激光后,所有激发的拉曼光和再通过可调滤波器为主的高光谱成像组件,成像在ccd上,可在几分钟内完成,以相元为单位,可以形成高达十万组拉曼光谱数据。是目前市面上*快的拉曼成像设备。
关键字:拉曼成像系统,高速拉曼成像光谱仪,激光拉曼成像光谱仪,高速拉曼光谱成像仪,拉曼成像高光谱,激光拉曼高光谱成像系统,激光拉曼高光谱成像仪,RAMAN imaging system,RAMAN spectrometer,RAMAN spectral system
RIMA拉曼显微高光谱成像系统
Photon etc公司RIMA拉曼成像技术是新一代快速、高精度、面扫描激光拉曼技术,它将共聚焦显微技术与激光拉曼光谱技术**结合,与传统的点成像拉曼系统不同,采用面成像技术,将激光扩束后,用特殊的光学元件将扩束后的高斯分布的激光整形成均匀分布的平顶激光,照射在样品上,滤除反射的激光后,所有激发的拉曼光和再通过可调滤波器为主的高光谱成像组件,成像在ccd上,可在几分钟内完成,以相元为单位,可以形成高达十万组拉曼光谱数据。是目前市面上*快的拉曼成像设备。
产品特点
1. 快速global mapping(非扫描式)
2. 百万像素拉曼光谱,成像时间仅几分钟
3. 斯托克斯和反斯托克斯
4. 高光谱分辨率和空间分辨率
设备原理图:
系统参数:
拉曼光谱测量范围
|
70 — 3200 cm-1
|
光谱分辨率
|
< 5 cm-1
|
空间分辨率
|
Sub-micron
|
显微镜
|
Inverted
|
物镜
|
20x, 60x, 100x
|
相机
|
Back-illuminated CCD camera, sCMOS或EMCCD
|
扫描速度
|
250 µm2/min at full spectral range
|
波长准确度
|
1 cm-1
|
激发波长
|
488,515,785 nm或者其他波长
|
应用领域:
纳米材料分析
Global Raman imaging is an exceptional technique for the analysis of
large surfaces of thin films and advanced materials. Its rapidity makes it a
great tool not only for universities and research institutes, but also for
industrial laboratories. With no or minimal sample preparation, RIMA™, Photon etc.’s new
hyperspectral Raman imager, can easily take part in routine analysis, where the
prompt access to information about sample composition is crucial for the
development of new materials.
With systems based on point-to-point or scanning technologies, the
acquisition of maps of large areas is often tedious and time consuming: the
analysis of a sample may take hours. RIMA™ expedites in minutes the
acquisition of the whole area in the field of view, rendering full maps of a
sample with unmatched rapidity. In fact, the hyperspectral cube is built image
by image, along the spectral window of interest, with a spectral resolution
better than 7 cm-1. Since a spectrum is recorded for each pixel, it is
possible, with a 1024 x 1024 pixels camera, to collect more than one million
spectra without moving the sample. Moreover, the size of the maps can be as
large as 650 x 650 mm2, depending on the magnification of the objective used
for the analysis. Photon etc.’s filters used for hyperspectral imaging are
based on holographic gratings, and provide very high efficiency for an optimal
acquisition of the weak Raman scattering. Combined with top of the line low
noise CCD or EMCCD cameras, RIMA™ is the most efficient Raman imaging
system on the market.
In order to show the advantages of RIMA™ in the analysis of
nanomaterials in biological systems, carbon nanotubes (CNT) have been incubated
with a sample of Candida Albicans yeast cells and exposed to a
homogeneous (flat-top) laser excitation of 532 nm on the entire field of view.
With a 50X objective, an area of 260 x 130 μm2 was imaged, with a step of
4.5 cm-1 and an exposition time of 15 s. The complete analysis took 20
minutes, for a total of more than 60,000 spectra.
Figure 1 shows the Raman hyperspectral cube of a portion of the imaged
area containing the yeast. The monochromatic Raman images revealed the position
of the aggregated yeast cells stained with the CNTs. The typical signal of CNTs
(red line) confirmed their presence on the yeast cells, while in other areas
the hyperspectral camera did not detect any CNT Raman signal (blue line).
Raman Multiplexing
DEVELOPMENT
AND CHARACTERIZATION OF CARBON NANOTUBE BASED RAMAN NANOPROBES BY RAMAN
HYPERSPECTRAL IMAGING: MULTIPLEXING AND BIODETECTION
The potential of
Photon etc. Raman Imaging Platform, RIMA™, was demonstrated by
Pr. R Martel’s group at Université de Montréal in a recent publication in Nature Photonics on the development
of Raman nanoprobes [1].
These new kind of nanoprobes are based on single-wall carbon nanotubes
and J-aggregated dyes, such as α−sexithiophene (6T), β-carotene (βcar) and
phenazine (Ph). Compared to fluorescent probes, Raman probes have the
advantages of being more stable over long periods of times (weeks and years)
and they produce a unique signature with narrow peaks that allows easy
multiplexing of 3 probes or more using the same excitation laser energy. This
nanomaterial shows a very high Raman scattering cross-section, without any
photobleaching or fluorescence background, even at high laser intensities.
In this work RIMA™ enabled the imaging and multiplexing of
three different probes with sensitivity down to the single object as seen in
Figure 1. The different probes were deposited on a SiOx/Si surface and
characterized by taking a single hyperspectral image. We were able to
determine, without a doubt, the position of each isolated probe (diameters: 1.3
± 0.2 nm), and even identify the co-localized probes (Fig 1b, Ph and βcar). The
sensitivity, efficiency and hyperspectral properties of RIMA™ were essential to
the development of these probes.
The carbon nanotube, which serves as a capsule for the probe, can be
covalently functionalized to selectively target biomolecules, such as
streptavidin. We demonstrated RIMA™’s potential in the detection of probes
in a biological context by imaging the βcar probe functionalized with
PEG-biotin groups that targeted streptavidin.
A pattern of 10 μm spots of streptavidin was created by microcontact
printing and then incubated with the probes. The pattern was maintained hydrated
under a cover slip during imaging and the probes were detected where
streptavidin was located. Figure 2 shows Raman hyperspectral images at 1520
cm-1 of two printed surfaces, where streptavidin was deposited either
inside (main figure) or around the dots (inset). With a single acquisition, a
sample area of 133 x 133 μm2 was studied using RIMA™ with laser excitation
at 532 nm. Damages to the samples were also limited due to a uniform
illumination over the portion of the sample in the field of view. In terms of
spectral resolution and large surface area imaged, RIMA™ provided
hyperspectral images in a much shorter time then conventional point-by-point
mapping Raman imagers.
Raman hyperspectral imaging is a powerful technique to study a wide
range of materials, from nanopatterned surfaces to biological systems. Because
of its high throughput, RIMA™ allows the acquisition of spectrally
resolved maps of large area samples, without damaging the surface.
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