Tissue Engineering And Nanotheranostics

“9.61x6.69” b2815 Tissue Engineering and Nanotheranostics

Plasmonic Nanoparticles Application in Biosensor and Bioimaging 167

that it provides high contrast images and makes it possible to collect

the scattering light of plasmon nanoparticles at the singleparticle

level. To date, DFM is widely utilized to monitor biological events,

such as protein association and overexpression. Many modifications to

the conventional darkfield system like employing different illumina

tion methods, light sources and various CCDs, have been developed

to improve the signal and time resolution of DFM to identify single

molecular binding events.

4.1. Conventional Dark-Field Microscopy

In a typical DFM system, the white light of a Halogen lamp pass

through a condenser to tilt the incident illumination and are focused

at the sample to excite the plasmons. The condenser is equipped with

a circular block at the lens to permit light with high angular transmit.

Most of the light is directly transmitted through the sample and is not

collected by the objective below the stage because the numerical aper

ture of objective is smaller than the condenser, causing the dark back

ground. Only the scattered light from the sample could be collected

to image sample in truecolor or to analyze single particle spectra.

4.2. Improvements in Sensitivity and the Speed of

Dark-Field Microscopy

The main limitation of conventional DFM is the low signal intensity

for nanoparticles smaller than 50 nm. To obtain sufficient SNR of

single nanoparticle, an intense light source and long recording time

(up to seconds) are both required, which makes DFM in suitable for

fast dynamic observation. To improve SNR and the temporal resolu

tion, several optical modifications have been developed. Noji et al.

developed the objectivetype evanescent illumination DFM by simply

replacing the dichroic mirror with a perforated mirror in a

conventional microscope.^13 In this system with total internal reflec

tion (TIR)illumination, the incident laser is reflected at the water–

glass interface and forms the evanescent field on the coverslip surface.

The evanescent field induces the oscillating dipoles within the

Tissue Engineering And Nanotheranostics

that it provides high contrast images and makes it possible to collect

the scattering light of plasmon nanoparticles at the singleparticle

level. To date, DFM is widely utilized to monitor biological events,

such as protein association and overexpression. Many modifications to

the conventional darkfield system like employing different illumina

tion methods, light sources and various CCDs, have been developed

to improve the signal and time resolution of DFM to identify single

molecular binding events.

4.1. Conventional Dark-Field Microscopy

In a typical DFM system, the white light of a Halogen lamp pass

through a condenser to tilt the incident illumination and are focused

at the sample to excite the plasmons. The condenser is equipped with

a circular block at the lens to permit light with high angular transmit.

Most of the light is directly transmitted through the sample and is not

collected by the objective below the stage because the numerical aper

ture of objective is smaller than the condenser, causing the dark back

ground. Only the scattered light from the sample could be collected

to image sample in truecolor or to analyze single particle spectra.

4.2. Improvements in Sensitivity and the Speed of

Dark-Field Microscopy

The main limitation of conventional DFM is the low signal intensity

for nanoparticles smaller than 50 nm. To obtain sufficient SNR of

single nanoparticle, an intense light source and long recording time

(up to seconds) are both required, which makes DFM in suitable for

fast dynamic observation. To improve SNR and the temporal resolu

tion, several optical modifications have been developed. Noji et al.

developed the objectivetype evanescent illumination DFM by simply

replacing the dichroic mirror with a perforated mirror in a

conventional microscope.^13 In this system with total internal reflec

tion (TIR)illumination, the incident laser is reflected at the water–

glass interface and forms the evanescent field on the coverslip surface.

The evanescent field induces the oscillating dipoles within the

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Tissue Engineering And Nanotheranostics

that it provides high contrast images and makes it possible to collect

the scattering light of plasmon nanoparticles at the single­particle

level. To date, DFM is widely utilized to monitor biological events,

such as protein association and overexpression. Many modifications to

the conventional dark­field system like employing different illumina­

tion methods, light sources and various CCDs, have been developed

to improve the signal and time resolution of DFM to identify single

molecular binding events.

4.1. Conventional Dark-Field Microscopy

In a typical DFM system, the white light of a Halogen lamp pass

through a condenser to tilt the incident illumination and are focused

at the sample to excite the plasmons. The condenser is equipped with

a circular block at the lens to permit light with high angular transmit.

Most of the light is directly transmitted through the sample and is not

collected by the objective below the stage because the numerical aper­

ture of objective is smaller than the condenser, causing the dark back­

ground. Only the scattered light from the sample could be collected

to image sample in true­color or to analyze single particle spectra.

4.2. Improvements in Sensitivity and the Speed of

Dark-Field Microscopy

The main limitation of conventional DFM is the low signal intensity

for nanoparticles smaller than 50 nm. To obtain sufficient SNR of

single nanoparticle, an intense light source and long recording time

(up to seconds) are both required, which makes DFM in suitable for

fast dynamic observation. To improve SNR and the temporal resolu­

tion, several optical modifications have been developed. Noji et al.

developed the objective­type evanescent illumination DFM by simply

replacing the dichroic mirror with a perforated mirror in a

conventional microscope.^13 In this system with total internal reflec­

tion (TIR)­illumination, the incident laser is reflected at the water–

glass interface and forms the evanescent field on the coverslip surface.

The evanescent field induces the oscillating dipoles within the

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Company

Features

Documentation

Resources

the scattering light of plasmon nanoparticles at the singleparticle

the conventional darkfield system like employing different illumina

collected by the objective below the stage because the numerical aper

ture of objective is smaller than the condenser, causing the dark back

to image sample in truecolor or to analyze single particle spectra.

fast dynamic observation. To improve SNR and the temporal resolu

developed the objectivetype evanescent illumination DFM by simply

conventional microscope.^13 In this system with total internal reflec

tion (TIR)illumination, the incident laser is reflected at the water–