In week 2 we built a simple light microscope and imaged neurons (fig 1). A glance at the image produced shows three key limitations of this approach: we lack contrast between our neuron of interest and the background; we observe a static readout of a dynamic structure; and we view the brain in slices, rather than in its complete form. A combination of fluorescence and genetic engineering have produced techniques to circumvent these limitations of microscopy.
Fluorescence
Fluorescent molecules absorb light of a given wavelength, which excites electrons into a high energy state. When these electrons relax, they emit light at a different, but specified, wavelength. Fluorescence microscopy utilizes these molecules by shining light at their absorption wavelength, and detecting light at their emission wavelength. If these molecules can be confined only to cells of interest, this produces a nearly infinite contrast between the sample and the background. Confining fluorescent molecules to cells of interest can be done in many different ways, but in many cases it relies upon advances in genetic engineering.
Famously, green fluorescent protein (GFP) was first discovered in glowing jellyfish in Friday Harbor. When the molecule absorbs (blue) light with a wavelength of around 488 nm, it undergoes a conformational change and emits (green) light with wavelengths around 509 nm (see figure 1). Its potential for applications in biology became apparent when Douglas Prasher and Martin Chalfie managed to managed to clone its nucleotide sequence and to express it in E. Coli and C. Elegans 1994. In neuroscience, GFP fused with Calmodulin (CaM) has proven to be an excellent marker of neural activity: when calcium binds to this complex, it undergoes a conformational change, enabling the absorption of light at the excitation wavelength. This is extremely useful, as it provides us with a method for monitoring neural activity by observing calcium transients through a microscope.
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Figure 1. Emission and excitation spectra of our set-up. Because the emission and excitation spectra of GFP overlap (blue and green lines), we used filters whose transmission bandwidths are shown in transparent blue and green. Lastly, the dichroic mirror (black line) transmitted the emitted (green) light from the sample, while reflecting the blue excitation light from our photo diode. Filter transmission data were retrieved from thorlabs.com and GFP excitation/emission spectral data from chroma.com.
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Designing the microscope
In order to exploit these properties of GFP for microscopy, the design of our microscope has to satisfy a few key characteristics that we summed up in figure 2.Firstly, to avoid contamination, we needed a way to make sure that there was no overlap between the light used for excitation and the light detected by our camera. As the excitation/emission spectra of GFP show some degree of overlap (fig 1), we placed a band-pass excitation filter in front of our LED light source to ensure only blue light (wavelength 469 ± 17.5 nm) would be sent into the sample. A green emission filter (525 ± 19.5 nm) was placed in front of our camera to ensure that all detected light came from fluorescence emitted by the sample, rather than from our LED. The emission filter undeniably discards much of the fluorescent light coming from the sample. However, since there is virtually no light that is coming from other sources than the sample, a very good signal to noise ratio can be maintained.
A second goal was to separate the paths of the excitation and the emission light. To achieve this, we placed a dichroic mirror between the tube lens and the objective. This dichroic mirror transmits light of wavelengths longer than 500 nm and reflects most of the light below that wavelength (figure 1), allowing us to avoid any excitation light hitting the camera.
A third, not entirely insignificant change to our microscope from week 2 entailed replacing the dismantled consumer webcam with a high-performance, highly efficient scientific CMOS camera. This camera has a quantum efficiency of 82%, meaning that 82% of the photons hitting the light-sensitive surface of the camera will produce an electric response.
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| Figure 2. Schematic representation of our fluorescence microscope |
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| Figure 3. The fluorescence microscopy set-up. |
Results
At the end of the week, we tested our fluorescence microscope by imaging zebrafish larvae that were provided by Elena Dreosti. These zebrafish expressed GCaMP, so that their neurons showed green fluorescence whenever the calcium concentration in their neurons increased. The fish were fixed in a gel, such that they could not move, and we imaged their neural activity in vivo by using a 16x magnification objective that can be immersed in water.The results of this imaging can be seen in this video (turn on HD for better resolution):
Neural activity in zebrafish tectum from Jesse Geerts on Vimeo.
Conclusions
By using fluorescent proteins and a combination of different wavelength filters and a dichroic mirror, we were able to build a fluorescence microscope that overcomes many of the limitations we saw in week 2; capturing only green light ensured that all light that hit our camera came from the neurons, solving most of our contrast problem. Moreover, this meant that we were able to look at a zebrafish brain in vivo and in real time, which was a major improvement from the static readout from a brain slice.
However, our microscope has some disadvantages that become apparent when looking at the video; GFP is expressed also in neurons outside the focal plane, and the excitation light will also hit these neurons, and they will fluoresce as well. Our wide field of view captures this light, meaning that part of our signal is polluted with light from outside the focal plane. As we will see in the next blog, this problem can only be circumvented by looking at a single point in the sample at a time.
Figure 2) schematic depicting our planned experiment, with a Neuroseeker probe inserted roughly parallel with the deep layers of the auditory cortex.
Figure 3) A) 10s of raw traces with events crossing the threshold (dotted line) marked with a black circle. B) Each event in the same time window is shown as a raster plot, and the total number of spikes detected in each channel over the entire recording is plotted as a heat map in C.
Spike sorting
Modern analytical methods are far more sophisticated than our approach. In fact, spikes detected by multi-channel probes can be allocated to their neuron of origin on the basis of waveform shape (mostly amplitude), which varies as a function of distance and orientation from the probe (figure 4). The action potential outputs of hundreds of cells can, therefore, be simultaneously sampled and allocated to their neuron of origin. Analytical tools such as KiloSort <link http://biorxiv.org/content/early/2016/06/30/061481> now support the near real-time sorting of action potentials from hundreds of cells at once.
Figure 4) Schematic showing how single action potentials from two cells can be allocated to their cell of origin. Left shows what a region of electrodes might detect in response to a single cell positioned near the probe. Right shows how two cells of slightly different positions might appear. The spatiotemporal pattern of events on different channels can then be used to group similar events that are likely to arise from the same cell.
Joana sorted the spikes with KiloSort and found 62 different well-isolated neurons contributing to the data. An example of one of these identified clusters can be seen in the figure below.
Summary
Overall for this part of the course we managed to acquire some exciting data – the first obtained by the lab with this configuration of the NeuroSeeker probe. We didn’t manage to test out our auditory experiments yet but we nonetheless have plenty of spontaneous data to tackle, which has allowed us to explore both rudimentary and state-of-the art analysis methods.
Figure 1 - Schematic diagram of microscope[/caption]
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Figure 2 - Opening the components of the microscope. Left: Before. Right: After.[/caption]
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Figure 3 - Microscope setup[/caption]
Results
Having set up our system we attempted to produce images from different samples at various magnifications. During testing and alignment, we used a slice of rat brain from Kampff lab. Our first successful production of an image can be seen in figure 4, where it is projected onto the forehead of SWC PhD student Jesse Geerts.
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Figure 4 - Image of a brain slice projected onto Jesse's head[/caption]
We next increased the magnification and replaced Jesse’s head with our modified webcam. As biological tissue can be hard to image, we tested our system by imagine a cloth, before moving onto imaging biological tissue (figure 5). We successfully imaged populations of neurons, and were able to identify a single neuron filled with biocytin (figure 6). We therefore succeeded in our aim of building a microscope capable of visualising neurons.
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Figure 5 - Left - Image of a cloth (left) and Nissl stained brain tissue (right) at high magnification.[/caption]
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Figure 6 - Image of a biocytin filled neuron (denoted by arrow)[/caption]
Conclusions
By using a very simple configuration of lenses, in a relatively short period of time we made a microscope capable of visualising neurons and produce a digital image. With some minor adjustments we could adapt this microscope to use fluorescence, or with a different configuration of lenses produce a higher magnification.
By combining our low and high pass filters in series, we also aimed to produce a band pass filter, where only a range of signals between two frequencies is able to pass. With the right combination of resistors and capacitors, this will allow us to filter out all non-relevant signals above and below the frequency range for (neuro)physiological signals.
Operational amplifiers
The physiological signals we aim to measure have amplitudes on the order of $10-100\mu V$ (EEG) or 20 mV (EMG). Furthermore, we observed that the filters we built attenuate the amplitude of the signals even more, which means that amplification will be necessary. Therefore, the second aim of this week was to build an operational amplifier (op-amp).
The basic principle of electronic amplification is a circuit that makes clever use of the properties of resistors and transistors. In the circuit shown in the figure, a positive voltage is applied at $V_{CC}$, and a negative voltage is applied at $V_{EE}$. Since the resistor at the tail of the circuit is much larger than the two parallel resistors at the top, the current flowing through this circuit is determined by the potential difference and this large resistor (following Ohm's law). If the input voltages ($ V^+_{IN}$ and $V^-_{IN}$) are equal, this means the current flowing through both arms will be equal, and the voltage measured at $V_{OUT}$ will be 0. When either one of the input voltages surpasses the other, more current will flow through that transistor, causing the measured voltage on the contralateral side to rise. The measured signal $V_{OUT}$ thus reflects the amplified difference between the input signals:
$V_{OUT}=A(V^+_{IN}-V^-_{IN}) $,
where $A$ is the gain of the amplifier. It should be noted that the circuit shown in the left figure is the simplest, original example of a differential amplifier, and it is dependent on the two transistors having exactly the same properties. Therefore, modern amplifiers use more sophisticated circuits.
This gain, which is typically on the order of 100,000, can be regulated with a negative feedback loop as shown in the right figure above. When (a proportion of) the output voltage is applied back into $V^-_{IN}$, the amplifier will drive the output voltage to whatever level necessary to keep the differential voltage between the inputs to zero. Thus, when a voltage divider is used to apply a proportion of the output voltage to the $V^-_{IN}$ port of the amplifier, one can use the relative sizes of the resistors to adjust the gain of the amplifier:
$A = \frac{R_1}{R_2} $
Outstanding difficulties
At the end of the week, we tried to apply the information mentioned above to record some muscle activity using an EMG electrode and an op-amp with negative feedback. We displayed the output voltage on an oscilloscope, but observed mainly noise. Next week, we will attempt to build a more sophisticated circuit, using pre-amplification and filtering.
