Opticoli
The new age of optics: Producing biological lenses and lasers to improve microscopy
Project Description
Limitations of microscopy
Microscopes have been around for hundreds of years and the technology behind these devices has been quickly developing over the past centuries. Especially fluorescence microscopy was an essential discovery for us biologists, since we are especially interested in what processes occur inside the cell. A popular approach to image intra- and extracellular processes is to use fluorescent tags to track a molecule- or gene of interest in the cell. These fluorescent tags can be imaged under a fluorescence microscope, allowing us to trace molecules and gene expression in a cell.
This popular technique has been essential for cellular research over the past decade, and has helped us to find out several important basics of life. Even though most techniques are already very far developed, it is essential that we keep developing microscopy techniques even further. When we can image every process going on in the cell, we are able to use this for our own good. We can, for example, image the mode of action of a disease, and cure this. An example of a disease that has been studied for years but still not fully understood, is Alzheimer’s disease (Hardy & Selkoe, 2002). If we could tag all molecules in a brain cell and image them, we might find what exactly causes the disease and hopefully develop a treatment. Also synthetic biology in general benefits from a good understanding of the cell. When we can trace all enzymes involved in a certain process, for example the alcoholic fermentation in yeast, we can more easily modify genes of interest and optimize this pathway for an improved production of biofuels.
Unfortunately, microscopy hasn’t advanced that far yet. Though super-resolution microscopy is quickly developing, there are still several limitations that hinder a full visualization of the cell. At this point, the technology and knowledge of microscopy is not the biggest limit for making detailed images of the cell; it’s the cells itself. When using fluorescence microscopy, the limit of the resolution of the microscopy is the amount of photons that your sample emits. However, not all photons are observed by the detector of the microscope, simply because not all photons reach this detector and get lost in the noise of the detector (Heintzmann & Ficz, 2006). Especially in tracing low intracellular concentrations or high-speed cellular processes, the amount of photons emitted is low (Lakowicz, 2013). We aim to improve this limit of microscopy using synthetic biology.
Improving microscopy using biology
The chance of a photon being observed is defined by both the chance of the photon being emitted and the photon being detected (Heintzmann & Ficz, 2006). We have thought of two possible solutions to improve the observation of a photon. The first one is increasing the chance of a photon being emitted by the sample, which in this case, are our cells. We will do this by modifying the cells in such a way they are emitting more photons for the same amount of fluorophores. This technique is based on the working principle of a laser. Therefore, we will call these cells the Biolaser.
A second approach to increase the chance of a photon hitting the detector is by directing the photons towards the detector. An easy way to do this is to apply a layer of lenses over the detector to focus the light onto the detector. A layer of tiny lenses is also called a microlens array. However, these microlens arrays are hard to fabricate and their synthesis is harmful for the environment. Therefore, we will modify bacteria in such a way they will become lenses: the Biolenses.
Synthetic biology to produce biological lasers
In order to modify E. coli in such a way that it is able to emit laser-like light, we first need to understand how a laser works. A laser has three essential components: a gain medium, an excitation source and a reflective agent. The gain medium is a medium with the ability to fluoresce. This gain medium is surrounded by a reflective agent, such as a mirror. This gain medium gets excited by the excitation source, which could be either an electric pulse or an external light source. Once this gain medium gets excited, it will emit photons. Because the gain medium is surrounded by a mirror, the photons cannot escape the gain medium but will ‘bounce’ back. When one of these photons hits an excited fluorescent molecule, something remarkable happens. This molecule will release an exact copy of the incident photon. This process is called stimulated emission. The result is that the light gets amplified each time it passes through the gain medium. Therefore, with only a limited amount of fluorescent molecules we can emit a lot more light compared to ‘conventional’ fluorescence.
In this project, we will use synthetic biology to modify E. coli in such a way that the bacterium will be able to emit laser-like light. In order to do this, we have to translate two of the main components of a laser, the gain medium and the mirrors, to biological alternatives that E. coli is able to produce. For the gain medium this is easy. We can transform E. coli with fluorescent proteins that will form the fluorescent gain medium. The biological alternative for mirrors is slightly less obvious. However, we believe to have found the solution in the enzyme silicatein. This enzyme is able to synthesize polysilicate, a biological glass (Müller et al., 2008; Müller et al. 2003). By transforming E. coli with the gene for this enzyme, we can let the cells coat itself in a layer of glass that will reflect the photons emitted by the fluorescent proteins. As an excitation source we can simply use a laser to excite the proteins. A figure of our synthetic biology approach to create a biological laser can be seen in figure 4. This biolaser will be able to emit a higher number of photons compared to a cell that is merely fluorescent. Therefore, this cell will be useful in fluorescence microscopy, since even a cell with a low number of fluorophores is hypothetically able to emit a high number of photons. Therefore, this cell could be clearly imaged. Our parts, experiments and results can be found in the Experiments section
Synthetic biology to produce biological lenses
The second approach to capture more light in fluorescence microscopy is by focusing the photons onto the detector of the microscope. We will do this with lenses, since they have the ability to focus light onto an object, such as the detector of a microscope, which is schematically shown in figure 5.
In a microscope, applying this technique would mean that each photovoltaic cell of the detector gets a lens placed on it that will direct all light into each cell of the detector. This means we need a matrix, or “array”, of lenses that are only a few micrometres small. These ‘microlens arrays’ already exist, and have been shown to be a good technique to focus more light onto photovoltaic cells, including the detector of a microscope (Jutteau, Paire, Proise, Lombez, & Guillemoles, 2015). We will also use this technique. However, we will not use the conventional, chemically produced microlenses, since they are very costly and their production is difficult and bad for the environment (Nam et al., 2013). Therefore, we aim to produce our own, biological microlenses that will be much greener and environmentally friendly compared to the conventional microlenses. Furthermore, we will also apply our biological microlenses in applications, other than microscopy, where collecting light is important. One of these applications in which we will apply our biological lenses are solar cells, more information can be found on the practices page
So how do we aim to produce these biological lenses using synthetic biology? The approach is the same as for the biological lasers: we transform E. coli with the silicatein gene. This gene allows the cell to cover itself in glass, resulting in a glass sphere of only 1-2 µm small. We will test the optical properties of this glass sphere as well as its functionality as a microlens. Since the shape of lenses is of high importance, we will also research ways to manipulate the size and shape of the cells, enabling us to produce different shapes of microlenses. Also, since our biological microlens contains a core of live bacteria, we will look into ways to sterilize the lens. This way, our product will not harm the environment in any way. Our parts, experiments and results can be found in the Experiments section
Experiments and results
Expression of different fluorophores
Introduction
One of the essential components of a laser is a fluorescent agent. Since our aim is to produce a fully biological laser, fluorescent proteins are favourable. To this end, we initially selected four fluorophores with different emission wavelengths: GFP, mVenus, mKate and mCerulean. These fluorophores were reported to have an increased fluorescent intensity compared to their wildtype (Cormack et al., 1996; Nagai et al., 2002; Shcherboo et al., 2007; Rizzo et al., 2004).
Since mVenus, mKate and mCerulean did not exist in the iGEM registry yet, we constructed a brand new part for each of these fluorophores including strong constitutive promoter and RBS (parts K1890010 and K1890011). GFP, on the other hand, was present in a whole range of biobricks. However, to our knowledge, there was no single biobrick available containing promoter, RBS and terminators. Hence, we constructed a new biobrick containing all of the above using the existing part E0840, consisting of RBS, coding sequence and terminators. By means of PCR we amplified this biobrick with primers designed to add a promoter while mainaining the biobrick prefix and suffix. Not only did we express GFP under the strong promoter J23100, but also under less strong promoters J23113, J23117, J23105, and J23108. This way we were able to see the influence of promoter strength on fluorescent output (parts K1890020 to K1890024.
Experiments & Results
In order to characterize these biobricks before further use, the emission spectra of the fluorophores were measured. Additionally, their effect on cell growth was investigated.
Emission spectra of different fluorophores
Introduction
To assure the fluorophores were functional, the emission spectra were recorded at the given excitation wavelength.
Methods
Parts encoding the four different fluorophores, including promoter, RBS and terminators, were expressed in E. coli BL21. GFP, mVenus, mKate and mCerulean were all expressed under the same strong constitutive promoter, J23100. Additionally, parts were constructed with GFP under control of promoters with different strengths, in order to investigate the influence of different fluorophore concentrations.
All of the mentioned biobricks were expressed in E. coli BL21. After growing in LB medium to an OD600 of ~1, the cells were washed and resuspended in the same volume of PBS. Aliquots of 100 µL were put in a 96 well plate.
The emission spectrum of each fluorophore was determined by exciting at a given wavelength and measuring the output intensity at a range of wavelengths. Because of this, the emission at a wavelength too close to the excitation could not be measured. This can be seen in the figures, where the left half of the emission peaks could not be measured. Especially for mVenus, where the excitation and emission wavelengths are very close together.
Results and Discussion
Fluorophores expressed under strong constitutive promoterAs all fluorophores were expressed under the strong constitutive promoter J23100, they were expected to show a strong fluorescence without the need of induction. Figure 1 shows that this was the case for GFP, mVenus and mCerulean. mKate, however, did not show any fluorescent activity and was therefore not used in the subsequent steps of the project.
GFP expressed under constitutive promoters of different strengths.Not only did we express GFP under the strong promoter J23100, but also under less strong promoters J23113, J23117, J23105, and J23108.
For comparison, the emission was normalized by dividing by OD. All strains were measured in the same dilution, in order to make the results reproducible. The emission intensity is as expected, corresponding to the strength of the promoters. All fluorophore spectra were also recorded in a dilution more suited for their emission intensity and normalized by 1 (Figure 3). From this figure we can conclude that all GFP biobricks function properly.
Back to TopThe effect of expression of fluorophores on growth
Introduction
As consitutive expression can sometimes be hard on the cells, we investigated the effect of the different consitutive promoters on cell growth. In a 24 hour kinetic cycle alterating shaking at 37°C with fluorescence and optical density measurements, we investigated whether this was the case.
Methods
An overnight culture in eM9 medium was inoculated in fresh eM9 to an OD600 of 0.1 in a 96 well plate. The emission at 522 nm was measured every 15 minutes. Measurements were done in quadruplicate with pure eM9 as a blank.
Results and Discussion
Figure 1 shows the 24 hour measurement of optical density and fluorescence intensity. The final OD600 is approximately equal for all different strains, suggesting that the level of constitutive expression was not influencing the growth. Furthermore, fluorescence intensity drops after the exponential growth phase, suggesting that GFP is being broken down by proteases as a response to nutrient limitation. After this event, growth continues at a slower pace, while GFP activity keeps decreasing. All in all, constitutive expression of GFP does not seem to have a detrimental effect on cell growth during exponential phase.
Cells expressing mCerulean or mVenus, however, seem to be having a longer lag phase before exponential growth starts (Figure 2). Also, they reach a lower final OD600 than the ones expressing GFP. These fluorophores might be slightly harmfull for cell growth. Nonetheless, they do grow and exhibit fluorescence, so they can be used in further experiments.
Back to TopDiscussion & Conclusions
We were able to succesfully construct and characterize two biobricks with brand new fluorophores for the iGEM registry: mVenus and mCerulean. Both of them exhibit a bright fluorescence, which is useful in our futher experiments. To our knowledge there was no part available in the registry consisting of promoter, RBS, GFP coding sequence and terminator Therefore, we constructed five new composite parts to provide single complete biobricks for GFP expression. These new parts were characterized and show a bright fluorescence, according to their promoter strength. All in all, our new parts provide a ready-to-go expression device for green, yellow, or cyan fluorescence, which can be very usefull for future iGEM teams.
Coating the cell in polysilica using silicatein
Introduction
For both the biolaser and the biolenses we need a coating of polysilicate, biological glass, around the cell. For the biolaser this glass will form the cavity that will enable the cells to emit laser-like light. For the biolens, the glass will give optical properties for the cell. E. coli is intrinsically not able to coat itself in polysilicate. However, upon transformation of the silicatein-α gene, originating from sponges, it is possible to coat the bacterium in a layer of polysilicate (Müller et al., 2008; Müller et al. 2003). Therefore, we are transforming E. coli with silicatein-α. We test the use of two different silicateins, one originating from the marine sponge Suberites domuncula (Müller, 2011) and one originating from the marine sponge Tethya aurantia (Cha et al., 1999). We express the enzyme in three different ways. First of all, we expressed the gene from S. domuncula (Part K1890000) and see if the enzyme is transported outside the cell as described by Müller et al, 2008. Furthermore, we express a fusion of silicatein from T. aurantia to the trans-membrane protein OmpA (outer membrane protein A) from E. coli to anchor the silicatein to the membrane (Part K1890002) (Curnow, Kisailus, & Morse, 2006; Francisco et al. 1992), which might make coating the cell specifically in polysilicate more efficient. We also express a fusion of silicatein from S. domuncula to the transmembrane Ice Nucleation Protein (INP) from Pseudomonas syringae (Part K1890001), a popular protein for membrane fusions (Kim & Yoo, 1998). Using these different approaches we expect to coat the cell in polysilicate, an overview is shown in figure 1. This glass coating around the cell will be the basis of both our biolens and –laser.
Experiments & Results
To determine if we have successfully covered E. coli in polysilicate, and to characterize the properties of the silicate-coated cells, we have performed a series of tests. First of all, we have stained the cells with rhodamine, a fluorescent stain that is able to bind to polysilicate. These stained cells were observed under a fluorescence microscope to determine whether the polysilicate shell was present. Furthermore, the polysilicate-synthesizing cells were observed using both Scanning Electron Microscopy (SEM) and Transmission Electron Microscopy (TEM). We have also determined the physical properties using Atomic Force Microscopy (AFM) to see whether the polysilicate layer changes the stiffness of the cells. Lastly, we have also performed a growth study of the polysilicate-coated cells to determine whether the polysilicate layer affects growth of the organisms.
Rhodamine staining of silica covered cells
Introduction
After transforming E. coli with the different silicatein BioBricks, we wanted to confirm and image whether the cell had indeed synthesized a layer of polysilicate around itself. Before using any advanced imaging techniques, we first used a much simpler technique. It is possible to stain polysilicate depositions with the fluorescent stain Rhodamine 123. This stain has shown to bind specifically to polysilicate (Li, Chu, & Lee, 1989). Since the stain is fluorescent, we can image it with a simple fluorescence microscope. If a cell has a polysilicate layer, the Rhodamine will bind to it which we can image.
Methods
The experiment was performed using E. coli BL21 with the following plasmids and conditions. All genes are under an inducible promoter.
Plasmid(s) | IPTG | Silicic acid | Rhodamine 123 |
---|---|---|---|
OmpA-Silicatein | + | + | + |
Silicatein | + | + | + |
INP-Silicatein | + | + | + |
OmpA-Silicatein (negative control) | + | - | + |
OmpA-Silicatein | + | + | - |
The cells were stained with 0.1 vol% Rhodamine. And washed 5 times with PBS, prior to imaging in a fluorescence microscope at 488nm (Li et al., 1989; Müller et al., 2005). Both widefield- (light microscopy) and fluorescence microscopy were used to image the cells.
Results and discussion
The stained cells were first imaged at maximum excitation intensity. At this excitation energy, only OmpA-silicatein showed fluorescence specifically localized at the cells and not in the medium. Silicatein, INP-silicatein and the negative control (OmpA-silicatein without silicic acid) all caused overexposure of the camera. In figure 1 the imaging results of OmpA and the negative control (OmpA-silicatein without silicic acid) are shown. The cells that were not stained with Rhodamine showed no measurable fluorescence. (data not shown).
Since Silicatein, INP-silicatein and the negative control all caused overexposure of the camera, they all had the same output. We can thus not draw any conclusions for these strains. Therefore, samples where overexposure was observed were imaged again at only 1/3 of the excitation energy. The imaging results are displayed in figure 2.
From figures 1 and 2 we can see that the strain transformed with OmpA-silicatein clearly has a different output from the negative control (figure 1). The fluorescence is only localized at the cells. This might mean that the Rhodamine has stained these cells and therefore the OmpA-silicatein cells could have the polysilicate layer around their membranes. We cannot distinguish a clear difference between silicatein, INP-silicatein and the negative control (figure 2). The entire medium is fluorescent, which causes overexposure of the camera at high excitation intensity. This might mean that the Rhodamine is not specifically located at the cell walls, but still dissolved in the medium.
Because the cells were analyzed at different excitation energies, so different camera settings, it is impossible to draw a conclusion from solely the images. Therefore, we analyzed the pictures using ImageJ. We measured the intensity of the fluorescence of the cells and the intensity of the fluorescence from the background. Then we normalized the intensity of the cells over the intensity of the background (in this case, the medium). This way, the intensity of the background of all samples becomes 1 and the intensity of the fluorescent cells has a relative value to the background signal. With this method, we are able to compare the fluorescence intensities of the cells, despite the different camera settings. The results of this calculation are shown in figure 3.
In figure 3 we see that the fluorescence intensity of the OmpA-silicatein strain is significantly higher than for the the silicatein and INP-silicatein strains. The silicatein and INP-silicatein strains have a fluorescence intensity comparable to the intensity of the medium (the background intensity). The negative controls (no silicic acid added, measured at two intensities) have the same output as silicatein and INP-silicatein. Therefore, we can conclude that these strains are not able to synthesize a polysilicate layer. However, we can conclude that the E. coli strain transformed with the OmpA-silicatein plasmid is successfully able to synthesize a layer of polysilicate around its membrane.
Back to TopImaging of silicatein-expressing cells using TEM
Introduction
Electron microscopy is an imaging technique that can acquire images with resolutions far above the optical limit due to the small wavelength of electrons (Nellist, 2011). An electron gun forms an electron beam which is focused and accelerated by magnetic lenses. When the electrons reach the sample, there are several interactions possible with the sample (figure 1). These various interactions can be used for different techniques. We have used high-angle annular dark-filed transmission electron microscopy (HAAFD-TEM) to make an image of the sample, energy dispersive x-ray spectroscopy to analyze the element composition of the sample and scanning electron microscopy (SEM) to analyze the phenotype of the samples.
In HAAFD-TEM electrons pass through the sample and are inelastically scattered at a high angle and acquired by a detector. The amount of electrons scattered at a high angle depends on the thickness and the material of the sample. When the thickness is high, the sample scatters a lot it will appear bright in the image.
Energy dispersive x-ray spectroscopy (EDX) is an analytical technique to determine the elements present in the sample (Friel et al. ,2006). When the electron beam interacts with the sample x-rays can emerge from the sample. These electrons can be detected and are characteristic for the element which emitted the x-ray. In that way we can specifically determine which elements are present in our sample.
Methods
The experiment were performed using E. coli BL21 cells with the plasmid containing OmpA-Silicatein. Two samples were made where the first sample was induced with IPTG but no silicic acid was added and a second sample which was both induced with IPTG and silicic acid was added, therefore this sample will have a polysilicate layer. The samples were prepared by fixation using 1% polylysine on a quantifoil carbon grid.
Results and discussion
Both samples with and without silicic acid added were imaged using HAAFD-TEM and energy dispersive x-ray spectroscopy (figure 2). The cells are fixed at a Quantifoil carbon grid. In figure 2A and 2C the white structure is a cell laying on a hole in the grid. In each sample, we measured elemental composition of our sample including the silicon content (figure 2 B,D) the blue spots in these images indicate where silicon is detected. The grid itself already contains silicon but in the holes of the grid no silicon is present (figure 2 B,D). Therefore we measured the pressence of silicon in bacteria laying on a hole on in the grid to make sure we do not have background silicon signal from the grid.
For the sample where no silicic acid is added (figure 2 A,B), we can see some silicon present at the position of the cell. However, there is a significant increase in silicon detected for the sample where silicic acid was added to the sample (figure 2D). This shows that silicon co-localizes with the cell which means there is indeed a polysilica layer formed by the bacteria.
Back to TopImaging of silicatein-expressing cells using SEM
Introduction
The Scanning Electron Microscope, or SEM as it is called, is a widely used imaging technique in science. In SEM, a beam of electrons is accelerated by high voltage and it is directed towards the sample with speeds up to \( 1.64 \times 10^5 km\). When the beam hits the sample, x-rays, backscattered electrons and secondary electrons are generated. For imaging, SEM uses the secondary electrons. Those secondary electrons are then collected and their kinetic energy is transformed to an image. (Kwakernaak & Sloof, 2005) It is highly used due to its very high spatial resolution and Depth of Focus (DoF). SEM can reach resolution of 5 nm and DoF about 0.5 mm, compared to an optical microscope that can reach a spatial resolution of \( 0.2 \mu m \) and DoF \( 1 \mu m \). With SEM it is only possible to image solid samples because the measurements take place under vacuum.
With SEM, we hope to see the impact of the polysilicate layer on the phenotype of the cell. If we want to make microlenses, the surface of the cell should be smooth, despite the silicatein layer. Any deformations in the layer can cause optical aberrations. Since SEM has a very high spatial resolution, we can use this technique to image what our silicatein-covered cells look like and to see what effect the polysilicate layer has on the strains.
Methods
The polysilicate layer around the cells was prepared according to the polysilicate layer protocol. As a negative control, uninduces cultures (no IPTG) and cultures without substrate (no sodium silicate) were used. The samples were fixed with gluteraldehyde and imaged with SEM. We used an FEI Niva Nano 450 SEM, under high vacuum.
Results and Discussion
Figure 1 shows SEM images taken of samples in the presence (A, B) or absence (C, D) of silic acid.
First of all, since we know from the rhodamine staining experiment that the polysilicate layer is present, it does not seem to influence the cell shape. However, the cells that are expected to have a polysilicate layer appear to be somewhat fused together. According to Müller et al (2008), cells possessing a polysilicate layer appear to be fused by a viscous cover. This can, however, also be the result of limited imaging resolution. When using titanium oxide as a substrate, Curnow et al (2005) reported large aggregates visible by SEM. This was not observed in the current experiment. Therefore, we can conclude that the polysilicate layer does not form aggregated or influence the shape of the cell, but form a homogeneous layer around the cell.
Back to TopAnalysis of physical properties of silica covered cells using AFM
Introduction
The physical properties of polysilica are different then those of the cell. We wanted to determine how the physical properties of the cell changes when encapsulated by a layer of polysilica. Therefore we determine the stiffness of cells with and without a layer of polysilica using atomic force microscopy (AFM). The stiffness is the rigidity of the a material, describing how easy the cell is deformed.
AFM is a technique used to determine surface characteristics of a sample. In AFM a very sharp tip scans over the surface of the sample. While scanning over the surface every height change is detected by a laser which is reflected by the cantilever on a position-sensitive photodetector (Figure 1). We used the PeakForce QNM mode of AFM, in which also surface characteristics like the stiffness and deformation can be determined. The stiffness is computed from the relation between the force at which the cantilever pushes on the sample, the adhesion force and the deformation of the material.
Methods
Experiments were performed using E. coli BL21 cells transformed with the plasmid containing the OmpA-Silicatein gene and induced with IPTG. Silicic acid was added to one sample to form the polysilicate layer around the cell. Another sample with no silicic acid added was used as a control. The cells weres spun down and resuspended in MilliQ and fixated on a glass slide using 1% ABTES.
Results and discussion
We have imaged two samples with AFM. The first sample is OmpA fused with silicatein with silic acid added so that the cell can encapsulate itself with biosilica (figure 2A-B). The second sample, that wa used as a control, did not contain silicic acid (figure 2C-D). From both samples a height map (figure 2A,C) and the stiffness (figure 2B,D) was determined. Both samples were fixed on a glass slide in the same way. Due to a tip change is there a factor 10 difference between the stiffness of the glass slide of both samples.
Viability experiments of silica covered cells
Introduction
Since the silicatein expressing cells are to cover themselves in polysilicate, their nutrient supply might be limited by diffusion, which can eventually result in cell death. To investigate whether this is indeed the case,a growth study was performed.
Methods
Cells containing the three different silicatein biobricks were grown overnight in selective LB. They were transfered to fresh medium and grown until in exponential phase. Then IPTG was added to induce expression. After a subsequent incubation of three hours, the medium was supplemented with silicic acid as substrate for silicatein. During the following five hours samples were taken, of which a 10-6 dilution was plated on selective LB plates. Colony forming units (cfu) were counted the day after.
Results and Discussion
Cells expressing either silicatein (Sil), silicatein fused to INP (INP Sil) or silicatein fused to OmpA (OmpA Sil) were tested. As a negative control, OmpA Sil Taur expressing cells without silicic acid were used. After one hour no colonies were observed on the plates on which the cultures with silicic acid were plated (Figure 1). The cultures without silicic acid continued to grow until after five hours.
This figure suggests that either the polysilicate layer inhibits nutrient diffusion into the cell, unlike reported by Müller et al. (2008), or the sodium silicate has a detrimental effect on growth.
Back to TopDiscussion & Conclusions
In this part of our project we have transformed E. coli with a gene encoding the enzyme silicatein in three different ways. We solely expressed the silicatein protein, but have also fused the protein to two different membrane proteins, INP and OmpA. The goal was to let the cells produce a polysilicate layer around their membrane, so the cell was completely covered in this biological glass. We have characterized the polysilicate-covered cells by electron microscopy, AFM, fluorescent staining and with a growth study.
After staining the silicatein-expressing cells with the fluorescent stain Rhodamine 123, which binds specifically to the polysilicate layer, we found that the cells transformed with the OmpA-silicatein fusion successfully synthesized a polysilicate layer around the cell, therefore we continued all experiments with this strain. This result was confirmed with TEM and EDX spectroscopy, where a higher concentration of silicon was found on the polysilicate-synthesizing cells. SEM showed that this layer is a neat, homogeneous layer and does not form any aggregates of polysilicate on the cell. Aggregates could seriously disturb the optical properties of our cell, so it’s a good results that our cells are covered homogeneously. AFM showed that the cells covered in polysilicate have a higher stiffness compared to cells without the polysilicate layer. This proves the presence of this layer. The finding that the cells are more rigid is also useful for our idea to develop biolenses, since these should not easily break. Lastly, our growth study shows that the cells covered in polysilicate live shorter that cells without this layer. This means that when we want to produce microlenses at a high scale, we should first grow the cells prior to incubating them with silicic acid. The fact that the cells die when they are encapsulated could also make it easier to use our microlenses in user-products. Bringing GMO’s out of the lab is often not permitted, so if we can show that our biolenses are inviable, this would not be a problem for our product. So, from these expreiments we can conclude that we have successfully genetically modified E. coli in such a way that it covers itself in a homogeneous layer of polysilicate. We can use these cells for further experiments on their ability to function as a laser or lens.
Engineering a biological laser
Introduction
Our cellular laser consists out of two features: fluorophores will be the light of the laser and a silica layer synthesized by silicatein will be the ‘mirrors’ that reflect a part of the photons emitted by these fluorophores. The fluorophores first need to be excited by an external light source. This could be either an LED source or a conventional solid laser. For fluorescence an LED excitation source suffices. However, we want lasing to happen in our cells. For this to happen, we need ‘population inversion’, which means the majority of the fluorophores is in an excited state (Gather & Yun, 2011; Svelto & Hanna, 1976). More information on this can be found in the project description. In order to excite the majority of the fluorescent proteins at the same time, we need a strong excitation source. Therefore we need to use a laser to excite the fluorphores in our biolaser. However, a major downside to using lasers for fluorophore excitation is the occurrence of photobleaching (Eggeling, Widengren, Rigler, & Seidel, 1998). The laser power required for the excitation of fluorophores to induce population inversion in the cell is so high it will photobleach the fluorophores within microseconds (Jonáš et al., 2014). Therefore, we need a custom laser setup to prevent photobleaching but establish the population inversion required for our biolaser. This laser setup should contain a pulsing laser which pulses at a frequency that will maintain the excited state but does not photobleach the proteins.
The appropriate set-up was not available, so we decided to build our own microscope out of separate optical parts. By discussing our problem with optics- and photonics companies and showing our motivation to solve this challenge, we were able to get all our required components sponsored or borrowed, making the entire set-up nearly cost-free. With our minimal set of available tools, we calculated and designed the optics in such a way that we could image fluorescent cells, while photobleaching was minimized. After days of laser aligning, we managed to do so. More information on the design of this setup can be found on the hardware page.
Using our custom-built setup, we analysed our ‘Biolaser’-cells, to see if they were able to produce a laser-like emission of light.
Experiments & Results
The first and foremost experiment to be done with the setup was to image the cells in order to see if the setup works properly and to see whether we can image cells with it. Once we have confirmed that the setup works properly, we can measure the output intensity of the cells to see whether the cells are able to emit laser-like light.
Imaging our biolaser using our home-built setup
Introduction
Building an optical setup is a very precise work. First, it is important to calculate the positions of all components in such a way that the laser beam will reach your sample, and the light emitted by the sample consequently reaches the detectors of the camera and spectrometer. Once this is done, all optical components are positioned on an optical table. This special table is made to prevent vibrations in you system and has mounting holes so all optical components can be screwed into place. Once the components are positioned on the table, the alignment begins. In this step, the beam coming from the laser is guided throughout the system. By slightly adjusting and repositioning all optical components the light is guided through the components until it reaches the detector of the camera. It is essential that the components are aligned correctly and are free of vibrations, because this could change the path of the light.
After tens of hours of carefully placing components and aligning the light through the setup, we managed to direct the light from the laser, through all components onto the detector of the camera. However, this does not necessarily mean that when we add fluorescent cells to the setup it we are able to image the cells with the setup. Any error in the setup could cause it not to work. Therefore, we first had to confirm whether our setup was working.
Methods
In order to confirm whether the setup was working, we used E. coli BL21 cells that were transformed with our constitutive mCerulean BioBrick. In previous fluorescent plate reader experiments, we have confirmed that these cells are able to fluoresce and that they can be excited at 405nm, the wavelength of our laser. To make sure the only output we were measuring was fluorescence, and not any ‘leakage’ of light from our laser beam, we also tested cells that were not transformed with the mCerulean BioBrick. These cells are not able to fluoresce after excitation at 405nm, so if the setup is working properly we should not get a signal from these cells.
The cells were adhered to the microscope slides using 3% agarose pads and imaged at an excitation intensity of 0.5 mW. This energy is low enough to not instantly photobleach the proteins, but observe fluorescence clearly. Focusing on the cells was done manually with a 50x oil-immersed objective. The cells were excited with a Coherent OBIS LX 405nm laser and images were taken using a DeltaPix Invenio III CCD camera.
Results & discussion
Imaging the cells with the setup yielded the following results:
As we can see in figure 2B, the cells transformed with a gene for the fluorescent protein mCerulean are clearly visible. When using a strain transformed with a plasmid that is not known to cause the cells to fluoresce, in this case OmpA-silicatein, no light was observed, as shown in figure 2A. To confirm that this sample did contain cells, we also inspected the sample with light microscopy, as shown in figure 3.
In figure 3, we see that the negative control did contain cells, but we could not observe a fluorescent signal. From this we can conclude that we successfully built a setup that is able to observe and measure fluorescence in a cell. There is no leakage of light of our excitation laser in the camera, since we do not observe anything when we use non-fluorescent cells. Also at a higher excitation energy (50 mW) we did not observe anything on the camera. Therefore we can conclude that our setup works as expected as it is indeed able to measure fluorescence without measuring other light sources.
For this experiment we used E. coli transformed with OmpA-silicatein that was induced and incubated in silicic acid, so it would contain the silica layer. We deliberately used this strain to test whether the silica or the cells had any autofluorescence that could interfere with our laser experiments. We did not observe any fluorescent signal for these cells, so we can conclude that the silica layer does not have any autofluorescence at 405 nm. Therefore, these cells are suitable for the laser experiments.
Back to TopIntensity measurements of laser cells
Introduction
One of the biggest differences between a laser and fluorescence is the amount of emitted photons. We can measure the amount of emitted photons by measuring the intensity of emitted light. The intensity of fluorescence increases linearly with the excitation energy. However, at a certain excitation energy it will reach the so-called ‘laser threshold’ and stimulated emission, and thus lasing will occur. From this point on, the output intensity of the fluorophores will still increase linearly, but with a much steeper slope, as shown in figure 1.
We investigated whether we could find the same relation between input and output intensity for our Biolaser cells, using our self-built setup, to investigate whether our cells were able
Methods
For this experiment we used E. coli BL21 transformed with the following BioBricks:
Plasmid(s) and conditions | Function |
---|---|
mCerulean (constitutively expressed) | Fluorescence |
mCerulean (constitutive) + OmpA-silicatein (induced, incubated in silicic acid) | Biolaser |
OmpA-silicatein (induced, incubated in silicic acid) | Negative control (no fluorescence) |
The cells were fixated on a microscope slide using 3% agarose pads. The cells were excited at a wavelength of 405 nm. The cells were imaged at excitation energies of 0.1 mW, 0.5 mW, 0.7 mW, 1 mW, 2 mW, 5 mW, 10 mW and 50 mW. These images were analysed using ImageJ to determine the output intensity and corrected for background noise (McCloy et al., 2014).
Results and discussion
The output intensities of our cells were plotted against the excitation power to determine whether our cells emitted laser-like light. The results are shown in figure 2.
In figure 2, the measured intensity is plotted against the excitation power (black dots). Since we expect a linear relation, the expected increase of intensity of fluorescence (blue line) and the expected increase of intensity for lasing (red line) was also plotted. Comparing the measurement data to the expected relations, we can not see a convincing result that our cells are lasing. Above an excitation power of 2 mW we see that in all cases the fluorescence stays at the same level. This means that the intensity is not increasing anymore and we observe photobleaching. So, both the fluorescent cells as well as the laser cells do not emit any laser-like light. For the fluorescent cells that were transformed with solely mCerulean, this result is as expected, these cells do not have any extra modifications that should cause them to emit laser light. The strain that was transformed with both mCerulean and OmpA-silicatein had a glass shell around the cell that could cause the cells to emit laser light. This effect was not observed. The strain transformed with solely OmpA-silicatein did not emit any light, as expected.
From this experiment we can not see any clear proof of lasing in our cells. This could be both due to our setup or due to the constructed cells. Previous studies show that lasing susually occurs at an excitation power under 1mW (Gather & Yun, 2011; Fan & Yun, 2014). However, up to this excitation power the Biolaser cells follow the same slope as the fluorescent cells, which means that no lasing occurred. From 2 mW and higher the cells bleach. Since we expected the cells to lase at an excitation energy under 1 mW, we did not take such high energies into account while designing our setup. Even though we exposed the cells to the excitation laser for a very short time, the power was probably so high that the cells eventually photobleached anyway.
Even though the excitation laser eventually bleached the fluorophores, this was probably not the reason why lasing didn’t work. Lasing should have occurred at an excitation energy between 0 and 1 mW, and at these energies the fluorophores did not bleach. It is possible that our cells were lasing at the low energy prior to bleaching, but the system was not sensitive enough to measure this. However, we did find a more probable reason why the cells did not lase. Modeling showed, that in a cavity as big as E. coli (around 1 µm) we need an intracellular fluorophore concentration of 0.1 M to get lasing. In our cells the maximum concentration we can achieve is in the nM to µM range and therefore lasing physically not possible in our cells. To get lasing, we would either need much larger cells or a much higher concentration of fluorophores. Therefore, it was most likely not due to the self-built setup nor our synthetic biology design of a biolaser that we did not observe lasing.
Back to TopDiscussion & Conclusions
We have successfully calculated, designed and built a custom optical setup that could allow us to measure lasing in cells. Using this self-built setup, we were able to image fluorescent cells and measure the intensity of the fluorescence. We have confirmed that the setup worked. We also measured if we got lasing in our fluorescent mCerulean polysilicate-covered cells. Despite the effort, we did not observe any lasing in cells. Our models have shown that this is due to the size of our cells, if we would use a bigger organism, e.g. a mammalian cell line, we could be able to measure lasing. Unfortunately, we were not able to measure this in our setup, since we did not have the safety permit to use mammalian cells. However, this would be a very interesting future study.
Engineering biological lenses
Introduction
Introduction on lenses & experiments
Experiments & Results
Introduction on the experiments that we did
Influencing cell shape for round lenses
Introduction
When making biological lenses, the shape of the lens is of crucial importance. E. coli is a rod-shaped organism, so it’s not symmetrical along all axes. Shining light on the round parts of E. coli has a different effect on the focusing of light than shining light on the long sides, see figure 1. More information on this can be found on the modeling page.
When we want to use our microlenses in more advanced optical systems, such as microscopes or cameras, we need to make sure that the variation between the different lenses is minimized. Manufacturers of optical systems do not accept a high aberration between different lenses, so it’s crucial for us to be able to control the shape of our lenses. We have decided to engineer E. coli in such a way that it becomes spherical. This way we are able to create spherical lenses. Apart from the fact that it is crucial to be able to control cell shape, round cells offer the advantage of being symmetrical along all axes, so the orientation of your lens does not matter for the optical properties.
In order to create spherical E. coli, we overexpress the BolA gene. BolA is a gene that controls the morphology of E. coli in the stress response (Santos, Freire, Vicente, & Arraiano, 1999). By overexpressing this gene at 37°C, the rod-shaped E. coli cells, will become round (Aldea, Hernandez-Chico, De La Campa, Kushner, & Vicente, 1988). We will express this gene both under a constitutive promoter (Part K1890031), as well as an inducible promoter (Part K1890030). When we express both the BolA gene as well as silicatein, we are able to construct round cells, coated in glass.
Methods
The expected phenotype of the cells expressing BolA is very different from the phenotype of wildtype E. coli. If the gene is successfully overexpressed, the cells become round, which we can easily observe under a widefield microscope. In widefield microscopy, the whole sample is simultaneously illuminated using a white light source so the phenotype of the sample can be inspected. This is comparable to normal light microscopy.
In order to obtain round cells we tested transforming E. coli BL21 with BolA under both an inducible promoter (Lac) and a constitutive promoter (J23100). Furthermore, we tried if transforming a strain with both BolA and the OmpA-silicatein fusion plasmid yielded round, glass covered cells. The following strains and conditions were tested under the widefield microscope:
Plasmid(s) | IPTG | Silicic acid |
---|---|---|
OmpA-silicatein (inducible) | + | + |
Lac-BolA (inducible) | + | - |
J23100-BolA (constitutive) | - | - |
OmpA-Silicatein (T. aurantia) + Lac-BolA (inducible) | + | + |
The cells were heat-fixed on a slide and observed under the widefield microscope at 37°C, Presence of the silicatein layer on the BolA cells was confirmed with Rhodamine staining which was imaged using fluorescence microscopy at 488 nm. Furthermore, imaged E. coli with and without the BolA-gene (induced) under SEM. The samples were fixed with gluteraldehyde and imaged with SEM. We used an FEI Niva Nano 450 SEM, under high vacuum.
Results and discussion
The four different strains were imaged under the widefield microscope, the taken images are shown in figure 2.
In figure 2, the widefield images of the four tested strains are shown. In figure 2A we can see cells with the characteristic wildtype E. coli phenotype; the cells are rod-shaped. Figure 2B shows that induction of the cells transformed wil BolA under the inducible Lac-promoter indeed has changed the phenotype of the cell. The cells have clearly become spherical. Constitutive expression of the BolA gene, as shown in 1C has the opposite result: the cells are rod-shaped and elongated. This is probably because of the stress the plasmid puts on the cells. As mentioned before, BolA is a gene involved in the stress response of E. coli that changes the morphology of the cells. A too high expression of the gene could therefore change the morphology in an unexpected way, such as elongation, a phenomena that is often observed in E. coli (Höltje, 1998). Since we require sphere-shaped cells, constitutive expression of the BolA-gene is not desired. Co-expression of the OmpA-silicatein fusion plasmid and the inducible BolA plasmid also yielded round cells, as seen in figure 2D.
We have confirmed the presence of the polysilicate layer around the cell using Rhodamine 123 staining, as shown in figure 3.
In this picture the cells do not look spherical, since the cells were imaged at room temperature, and BolA becomes active at 37°C. However, we have previously shown that these cells are capable of becoming spherical. In figure 3, we see a high fluorescence signal located at the cells, which means the cells also contain the polysilicate layer.
To get a more detailed view of the shape of the cells transformed with BolA, we also imaged the cells using SEM, the results are shown in figure 4.
In figure 4, we see that the cell shape of the cells transformed with BolA is indeed more spherical than the wildtype phenotype of E. coli. Also, we see that the size of the cells increased. Using ImageJ we analyzed the average size of 10 cells:
Phenotype | Average length (µm) | Average diameter (µm) |
---|---|---|
Wildtype | 1.2 +/- 0.12 | 0.5 +/-0.04 |
BolA | 1.0 +/- 0.15 | 0.87 +/- 0.13 |
In the table we see the average diameter of the cells increased. The average size of microlenses is in the order of tens or hundreds of micrometers, because with current techniques it's difficult and costly to produce smaller microlenses (Krupenkin, Yang, & Mach, 2003). The average sizes of photodetectors are in the nano- to micrometer range (Yang, Shtein, & Forrest, 2005). Our spherical microlenses approach this size, and are therefore usefulm since you could place one microlens over one photovoltaic cell, increasing the efficiency of the photovoltaic cell.
So, by inducing the expression of BolA, we are indeed able to control the shape of E. coli and turn the cell into a sphere. Also, transforming a cell with both silicatein-OmpA and BolA yields round cells, so the formation of the glass layer does not distort the cell shape. Rhodamine staining confirms the presence of the polysilicate cell. We have also shown that even though cell size increases upon expression of BolA, the size of our biolenses is smaller than the size of conventional microlenses. People have not been able to produce such small lenses in a cost-effective way, so our microlenses could be a possible solution to this.
Being able to control cell shape is of major importance if we want to create biological lenses, since the lenses are desired in various sizes and shapes. Especially spherical lenses are useful since they are symmetrical and therefore do not require a specific orientation; they will focus the light in the same way whatever their orientation is. From figure 2 we can see that the cells are not perfectly homogeneously shaped, there is some variation between the shape of the different cells. This variation is even clearer for the cells that contain the silica layer. This is possibly because two plasmids with a lac promoter put a great strain on the cells, resulting in a greater variation. For precision optics, it is extremely important that there is little to none variation between the lenses. Therefore, it’s recommended to do more research in controlling cell shape. However, since there is always a variation in gene expression between cells it will be wiser to conduct research into selecting or sorting the cells on their size or shape. A possible solution could be sorting the cells using FACS. As a future experiment, we could stain the silica-coated cells with Rhodamine and let a FACS-machine sort the cells on their phenotype.
Back to TopSterilization of the biolenses
Introduction
We wanted to test our biolenses in a real-world application: solar cells. This was chosen, since it was shown to make solar cells more efficient while using microlenses (Jutteau et al., 2015). Solar panels are currently unable to use all available solar energy, since parts of the light is lost due to non-focused beams. To decrease the losses, light needs to be focused, which can be done by lenses. Jutteau had shown already that solar panels are increased in efficiency while using microlenses. However, these microlenses are chemically produced, meaning under harsh environmental conditions. A high temperature combined with low pressures and harmful chemicals to produce these microlenses do not contribute positively in the total image of “environmentally friendly”.
In our opinion, the eventual product – microlenses – was promising. However, the production method did not add up with the purpose of increasing the potential of solar energy and thereby making general energy use more environmentally friendly. Our biologically produced E. coli cells covered in silicate were produced under physiological mild conditions (37 ºC, 1 atm and no harsh chemicals) and would fit much better in the image of environmental friendliness.
To put our cells to the test and see if these are just as promising in increasing the efficiency of solar cells as chemically produced microlenses, we have called for help in the department Photovoltaic Materials and Devices at the TU Delft. Here, prof. Dr. Arno Smets, had introduced us to Stefaan Heirman, a technician at the same research group. Stefaan helped us in our solar cell experiments.
Since Stefaan, including the to be used solar simulator and all other necessary equipment were at another faculty of the TU Delft, our cells had to leave the ML-1 lab. Here, safety regulations from the executed practices were incorporated in the labwork, since the biolenses should be outside the lab – into the environment as well as soon as they could be used on solar panels. Even though the growth study of our in silicate covered E. coli cells did not show any growth anymore after 1 hour, due to safety regulations we have decided to used an additional method to sterilize our biolenses.
To sterilize, different options are available. For example alcohols, chlorine and chlorine compounds are used within healthcare and autoclaving is a much-used method in laboratory settings. Besides that, UV sterilization is a much-used method in water treatment (Chang et al., 1985; Hijnen et al., 2006; O’Flaherty et al., 2016). This is used to remove among others E. coli. Since we do not want any chemicals to potentially interfere with our biolenses, we have chosen not to use any of these chemicals and to test whether autoclaving or UV sterilization would be a good option.
Methods
Autoclaving biolenses
Aliquots of E. colicells transformed with Sil_Sdom in pBbS5a were induced with silicic acid and subsequently autoclaved for 20 minutes at 121 ºC before imaged with scanning electron microscopy (SEM).
UV sterilization
For this experiment, E. coli cells transformed with BolA pBbA5c were used, as the results of the growth experiments just showed that cells covered in silicate were not viable. Since we did want a positive (absolutely living) control, we have chosen the BolA strain. For
A volume of 30 µL E. coli BL21 cells that were transformed with BolA in pBbA5c was plated on LB plates complemented with chloramphenicol. As controls for sterilization aliquots of 500 µL of the same cells were either heated at 95 °C for 10 minutes or washed with 500 µL 70% ethanol for three times. For UV sterilization, light bulbs emitting 254 nm were used and samples were exposed to it for 3 minutes. After sterilization, also 30 µL of these cells were plated on LB+Cm plates. Besides that, 30 µL of non-sterilized cells were plated as well. Of the last mentioned cells, it was expected for them to be alive and grow after overnight incubation.
Two of the plates containing BolA transformed cells were UV sterilized in a Stratagene UV Stratalinker 1800. The manufacturer recommended power settings of 120000 µJ. In our experiment we have used a power of 120000 µJ and 240000µJ to sterilize our cells.
All plates were incubated overnight at 37 °C.
Results
Autoclaving
Cells containing the Sil_Sdom gene were autoclaved and subsequently imaged with SEM.
Since the SEM showed the cells were collapsed, and in no way could function as biolenses, another sterilization method was used.
UV sterilization
To test the effectivity of UV sterilization on our E. coli cells, a growth study after UV sterilization was performed. For this 30 µL BL21 cells transformed with BolA in pBbA5c was plated on LB plates complemented with chloramphenicol. These plates were UV sterilized in a Strategene UV Stratalinker 1800. As positive controls the same cells were heated for 10 minutes at 95 ºC or washed three times with 500 µL ethanol. As negative control the same cells were plated on a selective plate.
Cell strain | Treatment | Number of colonies formed |
---|---|---|
BolA (pBbA5c) | UV sterilization: 120000 µJ | none |
UV sterilization: 240000 µJ | none | |
Heated 10 min at 95 ºC | none | |
Washed in ethanol | none | |
none | inf |
None of the sterilized plates showed any growth, while the non sterilized plate did yield colonies.
Now it was shown that the E. coli cells are not viable after UV sterilization, we also wanted to see the influence of UV sterilization on the physical properties of the silica layer. Since the silica layer already ensured unviability of the cells, UV sterilization could be seen as an extra safety precaution to compline to current synthetic biology safety regulations. For this, we have UV sterilized E coli cells transformed with Sil_Sdom, using 120000 µJ for 3 minutes and these were subsequently imaged with SEM (figure 2).
As shown in figure 2, the with silicate capturing of the cells remain undamaged after UV sterilization and could be used as biolenses now.
Discussion
In this experiment, different methods to sterilize our biolenses were tested, as we wanted to be able to put our biological microlenses in real-world conditions. For this, we have both autoclaved and UV sterilized our cells. From the growth study, it can be concluded that the biolenses were successfully sterilized by UV sterilization. Besides that, the shape of the biolenses was not affected by UV sterilization as opposed to autoclaving.
Back to TopImproving solar cells with biolenses
Introduction
The importance of measuring solar cell efficiencies
Solar panels are used to alter the potential of solar energy into electrical energy. A lot of innovation had already happened in this field, however the efficiencies can still use quite some improvement. As it was stated by Jutteau et al. (2015), the efficiency of solar cells could be increased significantly by adding a layer of microlenses. As parts of the available light get lost due to the fact that solar light is parallel and non-focused, the amount of electrical energy that can be retrieved from the sun could be higher. The focusing of the light can be solved however with lenses, as shown by Jutteau et al. (2015).
The microlenses used in this research are chemically produced, meaning under harsh conditions, such as an extremely high temperature, low pressure and harsh chemicals. This does, in our opinion, not complement the aim of being more environmentally friendly.
Our E. coli cells covered in silicate however, could form a biological alternative for these chemically produced microlenses. The biological microlenses, were produced under produced under physiological mild conditions (37 ºC, 1 atm and no harsh chemicals) and would fit much better in the image of environmental friendliness.
To put our cells to the test and see if these are just as promising in increasing the efficiency of solar cells as chemically produced microlenses, we have called for help in the department Photovoltaic Materials and Devices at the TU Delft. Here, prof. Dr. Arno Smets, had introduced us to Stefaan Heirman, a technician at the same research group. Stefaan helped us in our solar cell experiments. After sterilization, we visited Stefaan and compared efficiencies of solar cells using a solar simulator with and without our biologically produced microlenses.
Ways to measure the efficiency of photovoltaics
There are different ways to measure the output of photovoltaic (PV) cells with accuracy and repeatability. The most used characteristic of PVs is their efficiency (Power Conversion Efficiency or PCE). It is defined as the energy produced from the device by the intended radiation from a light source. In order to measure the efficiency and produce acceptable results; a set protocols were set in the scientific community.
Those protocols are relevant for the intended radiation and the measurements taken. For the intended radiation we make the assumptions of air mass 1.5 (dictates how the sun’s radiation is influenced by the atmosphere), the measured surface is 37 degrees from the equator and 48.2 degrees from Zenith. Finally, the radiation is 1000Wm-2 (Snaith, 2012) .
The parameters that influence the PCE measurements can be found in characteristic J-V diagrams, plotting current density (A/cm2) against voltage (V) (figure 1). The graph contains the three basic parameters of PCE measurements. Those are the short circuit current (Isc), the open circuit voltage (Voc) and the Fill Factor (FF). This graph is obtained by scanning the photovoltaic’s current output within a range of voltages, usually from -1 Volts to +1 Volts. The Voc is the voltage when the current is zero and the Isc is the current when the voltage is zero. The Fill Factor represents how much power the solar cell is producing or its theoretical maximum. The theoretical maximum power for each solar cell is \( P_{ideal} = V_{oc} \times I_{sc} \) and the maximum power is \( P_{max} = V_{max} \times I_{max}\) then the Fill Factor is defined as \(FF = \frac{P_{max}}{P_{ideal}} \). The Fill Factor is a defining term of the behavior of the solar cells (Grossiord, Kroon, Andriessen, & Blom, 2012).
Equipment and proposed measurements
In order to achieve those reproducible and accurate measurement of efficiency a certain type of equipment complemented with previously mentioned protocols need to be used. The equipment used to simulate the aforementioned conditions is called Solar Simulator, which is basically a big Xenon lamp with well-defined light power output. In order to calibrate the simulator a ‘standard’ cell is used with well-defined properties to measure the exact output of the simulator in each measurement. Finally, the tested device must be placed perpendicular to the light with nothing restricting the light path and not moved during the whole testing. Using this set of equipment, we are sure that we conduct all the experiments under the same scientifically accepted conditions so we remove a factor of uncertainty to our experimental results.
Methods
Results
Discussion
Back to TopDiscussion & Conclusions
Conclusion and discussion on the experiments
Conclusions & Recommendations
References
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