Difference between revisions of "Cell Imaging Using Picosecond Ultrasonics"

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(Related Publications and Talks)
 
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==Motivation==
 
==Motivation==
This project is to develop an instrument for imaging cells using their mechanical properties as a contrast mechanism. The goal is to produce a system that can be used as a general microscopy tool for cell biologists.
+
This project aims to develop an instrument for imaging cells using their mechanical properties as a contrast mechanism and with high resolution. The goal is to design and build a microscopy system that can be used as a general microscopy tool for cell biologists.
  
This is very challenging as to obtain high resolution imaging necessitates using high frequency ultrasound and at high frequencies the waves do not travel very far.  Picosecond laser ultrasound has been shown (link to bordeaux) to be a promising candidate.
+
To map the elasticity of cells with optical or higher resolution is very challenging. Ultrasound is a way to image with contrast derived from elasticity however, to obtain high resolution imaging this way necessitates phonons (GHz frequency ultrasound). To work at this regime poses many challenges: phonon generation requires laser light and heat which can damage cells,  at GHz frequencies the phonons do not travel very far and the pump-probe detection method is typically low in signal-to-noise ratio and slow in acquisition speed.  
  
==Detection mechanism - Brillouin Oscillations==
+
If all those challenges are solved, then there can be potentially greater benefits: the energy carried by phonons is orders of magnitude lower than that of light, which is suitable for live-cell imaging and allows to use arbitrarily small wavelengths for imaging leading to super-resolution. The contrast mechanism does not require the use of dyes so its label-free and of course it will provide means to image cells based on elasticity at a resolution never achieved before.
[[Image:Brillouin simple.png|150px|right]]
 
The  probe light is reflected from the sample surface to the detector, and if the sample is transparent there is also a reflection from the acoustic wave packet traveling in  the sample. This happens because the acoustic wave causes a change in  the local refractive index and so acts as a weak mirror.  These reflections interfere at the detector and as the phase of the  reflection from the acoustic wave is changing with time it leads to an oscillating  signal. These oscillations are termed Brillouin Oscillations.
 
  
The frequency ''F'' of the oscillation is given by the simple equation:
+
==Detection mechanism - Brillouin scattering in transmission==
''F = 2*Va*n/λ''
 
  
So if we can measure this signal we can measure the acoustic velocity ''Va'', as  long as we know the laser wavelength ''λ'' and the refractive index ''n''.
+
[[Image:Brillouin simple.png|250px|right]]
 +
 
 +
To solve some of the challenges of phonon imaging on cells, a novel detection configuration is being developed. In this configuration, an inverted microscope is used to deliver the pump and probe laser beams through the substrate where an opto-acoustic transducer converts pump light into a coherent phonon field while protecting the cells against unnecessary exposure to pump-light(UVA) and heat. The transmitted probe light (NIR) interacts with the generated phonon-field via Brillouin scattering which is collected and detected for imaging. Since the phonon field is propagating through the sample, its velocity and amplitude is related to the sample's elasticity. 
 +
 
 +
To detect the phonon field the scattered light interferes with the directly propagating light at the detector leading to an oscillating signal. These oscillations are termed Brillouin Oscillations and the Brillouin frequency ''f_B'' of the oscillation is given by the simple equation: ''f_B = 2*Va*n/λ'' which relates the acoustic velocity ''Va'' with the probe wavelength ''λ'' and the refractive index ''n''.
  
 
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<br style="clear:both" />
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|}
 
|}
  
The cells are grown on a transducer substrate similar to those described  [[Nanoscale_Ultrasonic_Transducers|here]]. The optimization of the  transducer layer is different in this case. Here we are much more concerned with optimizing the optical properties of the transducers. The  goal is to reduce the amount of blue light reaching the cell and either  maximize the reflected or transmitted light for the probe beam. We still have to ensure that the acoustic performance of the transducer is ok and that the acoustic bandwidth is sufficient to generate waves in the Brillouin frequency range of the sample.
+
The cells are grown on a transducer substrate similar to those described  [[Nanoscale_Ultrasonic_Transducers|here]]. The optimization of the  transducer layer in this case has the purpose to facilitate detection of Brillouin scattering in transmission and protecting the cells against pump light and heat. This is achieved by using an optical cavity/mechanical cavity as an opto-acoustic transducer. The cavity is designed to have maximum transmission at the probe wavelength while minimum at the pump wavelength. The cavity also is designed to resonate at the desired frequency for optimized SNR. Finally heat is managed through the use of a high thermal-conductivity substrate.
  
 
<br style="clear:both" />
 
<br style="clear:both" />
  
==Instrumentation advancements to enable imaging==
+
==Instrumentation ==
[[file:BNC_ASOPS_Layout.jpg|150px|right|alt=alt text|ASOPS pump probe instrument]]
+
[[file:BNC_ASOPS_Layout.jpg|250px|right|alt=alt text|ASOPS pump probe instrument]]
  
Measurements are made using a pump/probe picosecond laser ultrasound instrument utilizing ASOPS lasers. These laser control the delay between the pulse electronically removing the need to mechanically scan a delay line. this allows the very small signals present in these typos of experiments to be obtained quickly.  
+
Measurements are made using a pump/probe picosecond laser ultrasound instrument utilizing ASOPS lasers. These laser control the delay between the pulse electronically removing the need to mechanically scan a delay line. This allows the very small signals present in these typos of experiments to be obtained quickly.  
  
The pump beam is frequency doubled in a non linear crystal to have a wavelength of 390nm, the probe beam is at 780nm and both beams can be directed to the sample through and objective lens normal to the sample. optionally the pump beam can also be directed to the underside of the sample to generate the acoustic waves from below.
+
The pump beam is frequency doubled using a nonlinear crystal to give a wavelength of 390nm, the probe beam is at 780nm and both beams can be directed to the sample through and objective lens normal to the sample. optionally the pump beam can also be directed to the underside of the sample to generate the acoustic waves from below.
  
The instrument also has optical paths for wide field phase contrast imaging to allow the cells being studied to be visualized. This allows to assess the cells health and locate the scan region and register the acoustic image with the cell of interest.
+
The instrument also has optical paths for wide field phase contrast imaging to allow the cells being studied to be visualized. This allows us to assess the cells health and locate the scan region of most interest.
  
The acoustic signals are captured by recording the probe beam power with a photo-diode, this signal is then filtered and amplified before being digitized in a digital oscilloscope. To build up an image the sample is raster scanned.
+
The acoustic signals are captured by recording the probe beam power with a photo-diode, this signal is then filtered and amplified before being digitized with a digital oscilloscope. To build up an image the sample is raster scanned.
  
 
<br style="clear:both" />
 
<br style="clear:both" />
  
 
==Ultrasonic imaging of cells==
 
==Ultrasonic imaging of cells==
An example trace is shown below, there are three main components present in the signal.
+
An example of an experimental trace obtained using a glass substrate is shown below, there are three main components present in the signal: A signal from the transducer resonance, one from Brillouin oscillations in the glass, and one from the cell or media. These signals are all clearly separated in the the frequency domain as shown by the FFT.
A signal from the transducer substrate, once from Brillouin oscialltions in the glass, and one from the cell or media. These signals are all clearly separated in the the frequency domain as shown by the FFT.
 
 
{|class="wikitable" align=""
 
{|class="wikitable" align=""
 
|-
 
|-
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===Live Cells===
 
===Live Cells===
Measuring live cells is much more challenging, this is because the amount of light they can tolerate without being effected is much lower than the amount that would damage fixed cells. Secondly the cells can move around and so the scans need to be taken as quickly as possible.  
+
Measuring live cells is much more challenging, this is because the amount of light they can tolerate without being affected is much lower than the amount that would damage fixed cells. Secondly the cells can move around and so the scans need to be taken as quickly as possible.  
 +
 
 +
{|class="wikitable" align=""
 +
|-
 +
|[[Image:PLU_liveLineBrill2A.png |150px|alt=alt text|scan cell A]]
 +
|[[Image:PLU_liveLineBrill2B.png |150px|alt=alt text|scan cell B]]
 +
|[[Image:PLU_liveLineBrill2C.png |150px|alt=alt text|scan cell C]]
 +
|[[Image:PLU_liveLineOptical2_FluorAfter.png |300px|alt=alt text|Resonant Frequency]]
 +
|}
 +
 
  
The pictures below show a series of scans of live cells, their optical image and a corresponding fluorescence image which shows which cells are dead. if the cell is alive they do not fluoresce if they have died they light up.
+
{|class="wikitable" align=""
 +
|-
 +
|[[Image:PLU_Brillouin_mapl_exp2.png |150px|alt=alt text|scan cell A]]
 +
|[[Image:PLU_Himag_before_exp2.png |150px|alt=alt text|scan cell B]]
 +
|}
  
 
==3D imaging==
 
==3D imaging==
Line 97: Line 110:
 
|}
 
|}
 
Combining this map with the transition time information gives us the profile of the cell phantom.
 
Combining this map with the transition time information gives us the profile of the cell phantom.
 +
 
[[Image:PLU_phantom_profile.png  |400px|alt=alt text|trace of phantom cell]]
 
[[Image:PLU_phantom_profile.png  |400px|alt=alt text|trace of phantom cell]]
  
 
==Related Publications and Talks==
 
==Related Publications and Talks==
<bibtex>@article{smith_optically_2015, title = {Optically excited nanoscale ultrasonic transducers}, volume = {137}, issn = {0001-4966}, url = {http://scitation.aip.org/content/asa/journal/jasa/137/1/10.1121/1.4904487}, doi = {10.1121/1.4904487},}, number = {1}, urldate = {2015-02-09}, journal = {The Journal of the Acoustical Society of America}, author = {Smith Richard J. and Cota Fernando Perez and Marques Leonel and Chen Xuesheng and Arca Ahmet and Webb Kevin and Aylott Jonathon and Somekh Micheal G. and Clark Matt}, month = {jan}, year = {2015}, keywords = {Acoustic sensing, Optical resonators, Proteins, Ultrasonic transducers, Ultrasonography}, pages = {219--227},
 
</bibtex>
 
  
Richard Smith, Fernando Perez, LeonelMarques, Matt Clark,Design and application of nano-scaled transducers,Institute of Physics Optics + Ultrasound One Day Meeting, May 2013, Nottingham, UK
+
===Publications:===
 +
 
 +
'''Cell imaging by phonon microscopy: sub-optical wavelength ultrasound for non-invasive imaging'''. Fernando Perez-Cota et al, Imaging & Microscopy 2017 (3).
 +
 
 +
'''High resolution imaging of living cells with sub-optical wavelength phonons''' Perez-Cota F., Smith R. J. Moradi E., Marques L., Webb K, and Clark M. Scientific Reports.
 +
 
 +
'''Thin film transdcuers for subcellular Brillouin oscillation imaging of individual biological cells''', Perez-Cota F., Smith R. J. Moradi E., Marques L., Webb K, and Clark M.,Appl. Opts. 54 28 (2015)
 +
 
 +
'''Optically excited nanoscaled ultrasonic transducers''', Smith R. J. , Perez-Cota F., Marques L., Xuesheng C., Ahmet A., Webb K, Aylott J., Somekh M. G. and Clark M., JASA 137 1 (2015)
 +
 
 +
 
 +
===Proceedings:===
 +
 
 +
'''Cell imaging with sub-optical wavelength ultrasound'''. Clark M., Marques L., Moradi E.,Perez-Cota F., Smith R. J., and Webb K. Asia Communications and Photonics Conference (2015).
 +
 
 +
'''Thin-film transducers for the detection and imaging of Brillouin oscillations in transmission on cultured cells'''. Perez-Cota F., Smith R. J. Moradi E., Webb K, and Clark M.,JPCS AFPAC (2015)
 +
 
 +
'''Sound of nano''' J. Aylott, M. Clark, L. Marques, F. Perez-Cota, R.J. Smith and K. F. Webb. SPIE 8923, Micro/Nano Materials, Devices, and Systems Proceedings (2013).
 +
 
 +
 
 +
===Talks:===
 +
 
 +
Cell investigations using picosecond laser ultrasound imaging Perez-Cota F., Smith R. J. Moradi E., Webb K, and Clark M. '''LU Linz Austria (2016)''' oral presentation.
 +
 
 +
Cell imaging based on Brillouin oscillations detection in transmission using thin-film transducers Perez-Cota F., Smith R. J. Moradi E., Webb K, and Clark M. '''LU Chicago IL (2015)''' oral presentation.
 +
 
 +
Design and application of nano-scaled ultrasonic transducers F. Perez Cota, R.J. Smith, L. Marques, K. F. Webb and M. Clark. '''RCNDE ERS Glasgow (2014)''', oral presentation.
 +
 
 +
Nano-scale transducers for picosecond ultrasonics in living cells F Perez Cota, R. J.Smith, K. F. Webb and M. Clark. '''LU Yokohama Japan (2013)''' oral presentation.
 +
 
 +
Design and application of nano-scaled transducers R. J. Smith, F. Perez Cota, L. Marques, K. F. Webb and M. Clark. '''IOP Optics and Ultrasound day''' meeting at The University of Nottingham (2013), oral presentation.
  
Fernando Perez Cota, M. Clark, K. F. Webb, and R.J. Smith, Nanoscale transducers for picosecond laser ultrasonics in cells,3rd symposium of laser ultrasonics, June 2013, Yokohamma, Japan,
+
Nano-scale transducers for picosecond ultrasound in living cells F Perez Cota, R. J. Smith, K. F. Webb and M. Clark. '''AFPAC (2013)''' oral presentation.

Latest revision as of 11:02, 18 July 2018

Motivation

This project aims to develop an instrument for imaging cells using their mechanical properties as a contrast mechanism and with high resolution. The goal is to design and build a microscopy system that can be used as a general microscopy tool for cell biologists.

To map the elasticity of cells with optical or higher resolution is very challenging. Ultrasound is a way to image with contrast derived from elasticity however, to obtain high resolution imaging this way necessitates phonons (GHz frequency ultrasound). To work at this regime poses many challenges: phonon generation requires laser light and heat which can damage cells, at GHz frequencies the phonons do not travel very far and the pump-probe detection method is typically low in signal-to-noise ratio and slow in acquisition speed.

If all those challenges are solved, then there can be potentially greater benefits: the energy carried by phonons is orders of magnitude lower than that of light, which is suitable for live-cell imaging and allows to use arbitrarily small wavelengths for imaging leading to super-resolution. The contrast mechanism does not require the use of dyes so its label-free and of course it will provide means to image cells based on elasticity at a resolution never achieved before.

Detection mechanism - Brillouin scattering in transmission

Brillouin simple.png

To solve some of the challenges of phonon imaging on cells, a novel detection configuration is being developed. In this configuration, an inverted microscope is used to deliver the pump and probe laser beams through the substrate where an opto-acoustic transducer converts pump light into a coherent phonon field while protecting the cells against unnecessary exposure to pump-light(UVA) and heat. The transmitted probe light (NIR) interacts with the generated phonon-field via Brillouin scattering which is collected and detected for imaging. Since the phonon field is propagating through the sample, its velocity and amplitude is related to the sample's elasticity.

To detect the phonon field the scattered light interferes with the directly propagating light at the detector leading to an oscillating signal. These oscillations are termed Brillouin Oscillations and the Brillouin frequency f_B of the oscillation is given by the simple equation: f_B = 2*Va*n/λ which relates the acoustic velocity Va with the probe wavelength λ and the refractive index n.


Substrate Design

alt text alt text
alt text alt text

The cells are grown on a transducer substrate similar to those described here. The optimization of the transducer layer in this case has the purpose to facilitate detection of Brillouin scattering in transmission and protecting the cells against pump light and heat. This is achieved by using an optical cavity/mechanical cavity as an opto-acoustic transducer. The cavity is designed to have maximum transmission at the probe wavelength while minimum at the pump wavelength. The cavity also is designed to resonate at the desired frequency for optimized SNR. Finally heat is managed through the use of a high thermal-conductivity substrate.


Instrumentation

alt text

Measurements are made using a pump/probe picosecond laser ultrasound instrument utilizing ASOPS lasers. These laser control the delay between the pulse electronically removing the need to mechanically scan a delay line. This allows the very small signals present in these typos of experiments to be obtained quickly.

The pump beam is frequency doubled using a nonlinear crystal to give a wavelength of 390nm, the probe beam is at 780nm and both beams can be directed to the sample through and objective lens normal to the sample. optionally the pump beam can also be directed to the underside of the sample to generate the acoustic waves from below.

The instrument also has optical paths for wide field phase contrast imaging to allow the cells being studied to be visualized. This allows us to assess the cells health and locate the scan region of most interest.

The acoustic signals are captured by recording the probe beam power with a photo-diode, this signal is then filtered and amplified before being digitized with a digital oscilloscope. To build up an image the sample is raster scanned.


Ultrasonic imaging of cells

An example of an experimental trace obtained using a glass substrate is shown below, there are three main components present in the signal: A signal from the transducer resonance, one from Brillouin oscillations in the glass, and one from the cell or media. These signals are all clearly separated in the the frequency domain as shown by the FFT.

alt text alt text


Fixed Cells

By recording the Brillouin frequency while scanning the sample images can be taken. The below shows a Brillouin frequency map of a fixed fibroblast cell, this image shows the location of the nucleus (the redder region).

alt text alt text

A different fibroblast cell is shown below, here we can see much more detail, with the filopodia clearly visible.

alt text alt text

The image below shows a scan of a fixed cardiac cell, the striations of the cell are clearly visible, these repeating structures are how the cells contract, and have spacings on the order of a few microns.

alt text alt text


Live Cells

Measuring live cells is much more challenging, this is because the amount of light they can tolerate without being affected is much lower than the amount that would damage fixed cells. Secondly the cells can move around and so the scans need to be taken as quickly as possible.

alt text alt text alt text alt text


alt text alt text

3D imaging

It is possible to use signal processing techniques to extract more information from the data we obtain during the scans. By analyzing the frequency of the signal vs time we can extract changes in frequency with depth. This enables the mapping of internal structures in the cells, or should the acoustic waves leave the cell and enter the medium it allows us to obtain the profile.

There are a number of different ways to do this, from relatively fast and simple methods (zero cross analysis) to more complex approaches (wavelets).

Below is an example of the process for a phantom cell made from polystyrene beads. In the time trace the transition from the phantom back to the media is clearly visible.

alt text

If we take the Brillouin frequency map and a map of the refractive index we can produce a map of the acoustic velocity of the material.

alt text alt text alt text

Combining this map with the transition time information gives us the profile of the cell phantom.

alt text

Related Publications and Talks

Publications:

Cell imaging by phonon microscopy: sub-optical wavelength ultrasound for non-invasive imaging. Fernando Perez-Cota et al, Imaging & Microscopy 2017 (3).

High resolution imaging of living cells with sub-optical wavelength phonons Perez-Cota F., Smith R. J. Moradi E., Marques L., Webb K, and Clark M. Scientific Reports.

Thin film transdcuers for subcellular Brillouin oscillation imaging of individual biological cells, Perez-Cota F., Smith R. J. Moradi E., Marques L., Webb K, and Clark M.,Appl. Opts. 54 28 (2015)

Optically excited nanoscaled ultrasonic transducers, Smith R. J. , Perez-Cota F., Marques L., Xuesheng C., Ahmet A., Webb K, Aylott J., Somekh M. G. and Clark M., JASA 137 1 (2015)


Proceedings:

Cell imaging with sub-optical wavelength ultrasound. Clark M., Marques L., Moradi E.,Perez-Cota F., Smith R. J., and Webb K. Asia Communications and Photonics Conference (2015).

Thin-film transducers for the detection and imaging of Brillouin oscillations in transmission on cultured cells. Perez-Cota F., Smith R. J. Moradi E., Webb K, and Clark M.,JPCS AFPAC (2015)

Sound of nano J. Aylott, M. Clark, L. Marques, F. Perez-Cota, R.J. Smith and K. F. Webb. SPIE 8923, Micro/Nano Materials, Devices, and Systems Proceedings (2013).


Talks:

Cell investigations using picosecond laser ultrasound imaging Perez-Cota F., Smith R. J. Moradi E., Webb K, and Clark M. LU Linz Austria (2016) oral presentation.

Cell imaging based on Brillouin oscillations detection in transmission using thin-film transducers Perez-Cota F., Smith R. J. Moradi E., Webb K, and Clark M. LU Chicago IL (2015) oral presentation.

Design and application of nano-scaled ultrasonic transducers F. Perez Cota, R.J. Smith, L. Marques, K. F. Webb and M. Clark. RCNDE ERS Glasgow (2014), oral presentation.

Nano-scale transducers for picosecond ultrasonics in living cells F Perez Cota, R. J.Smith, K. F. Webb and M. Clark. LU Yokohama Japan (2013) oral presentation.

Design and application of nano-scaled transducers R. J. Smith, F. Perez Cota, L. Marques, K. F. Webb and M. Clark. IOP Optics and Ultrasound day meeting at The University of Nottingham (2013), oral presentation.

Nano-scale transducers for picosecond ultrasound in living cells F Perez Cota, R. J. Smith, K. F. Webb and M. Clark. AFPAC (2013) oral presentation.