Team:Newcastle/Modelling/CellShapeModel
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==Background== | ==Background== | ||
- | '''One of our research themes focuses on the ability of L-form bacteria to fit the mould and/or fill spaces by growing into them. We would like to explore the biophysical properties of the cell and the limits of the cell size the L-form can grow to before dividing by constructing a 2- | + | '''[https://2013.igem.org/Team:Newcastle/Project/shape_shifting One of our research themes] focuses on the ability of L-form bacteria to fit the mould and/or fill spaces by growing into them. We would like to explore the biophysical properties of the cell and the limits of the cell size the L-form can grow to before dividing by constructing a 2-dimensional cell model.''' |
- | The shape of the bacterial cell is usually determined by the structures of the cell wall and bacterial cytoskeleton. The cell wall of ''B.subtilis'' is a thick layer of peptidoglycan which contains cell-wall proteins, techoic and lipotechoic acids. Peptidoglycan is a rigid structure which helps to protect the cell from osmotic pressure and mechanical damage. It also helps the cell to maintain a constant shape, while not specifically defining it. This role is played by the cytoskeleton. The bacterial cytoskeleton is largely similar to that of eukaryotes. It is comprised of three types of protein structures: FtsZ, MreB and crescentin (only present in certain species) which are homologous to eukaryotic tubulin, actin and intermediate filaments respectively. These proteins also perform other functions in the cell; usually they are involved in cell growth and division and therefore are often essential for the cell's survival. The communication between the two regulatory components is assured by a series of membrane-associated enzymes (penicillin binding proteins). | + | The shape of the bacterial cell is usually determined by the structures of the cell wall and bacterial cytoskeleton. The cell wall of ''B.subtilis'' is a thick layer of peptidoglycan which contains cell-wall proteins, techoic and lipotechoic acids. Peptidoglycan is a rigid structure which helps to protect the cell from osmotic pressure and mechanical damage. It also helps the cell to maintain a constant shape, while not specifically defining it. This role is played by the cytoskeleton. The bacterial cytoskeleton is largely similar to that of eukaryotes. It is comprised of three types of protein structures: FtsZ, MreB and crescentin (only present in certain species) which are homologous to eukaryotic tubulin, actin and intermediate filaments respectively. These proteins also perform other functions in the cell; usually they are involved in cell growth and division and therefore are often essential for the cell's survival ([https://2013.igem.org/Team:Newcastle/Modelling/CellShapeModel#References Shih and Rothfield, 2006]). The communication between the two regulatory components is assured by a series of membrane-associated enzymes (penicillin binding proteins)([https://2013.igem.org/Team:Newcastle/Modelling/CellShapeModel#References Cabeen, Jacobs-Wagner, 2005]). |
- | + | ||
- | + | ||
- | + | ||
+ | Because L-forms lack the peptidoglycan cell wall, cells naturally adopt the most energetically favourable shape (i.e. sphere) regardless of the cytoskeleton structure. With protoplasts (cells with chemically digested cell wall), the growth, variation in shape and division is restricted due to the limited amount of the cell membrane which simply ruptures if the pressure inside the cell increases. The L-forms created with our BioBrick will have a mutation in the ''MurE'' gene which causes spontaneous increase in production of the ''IspA-like'' gene product which results in increased synthesis of the cell membrane. This stabilises the cell and allows for growth and division. | ||
==Approach== | ==Approach== | ||
- | For the purposes of the study the complex model of the growing cell inside of the confined space can be broken down to simpler models of the system | + | For the purposes of the study the complex model of the growing cell inside of the confined space can be broken down to simpler models of the system in three phases. The first phase would be a constantly growing cell, followed by a model of the cell when it touches the boundaries and therefore changes the trajectory of the membrane growth and finally starts adopting the shape of the boundaries. |
===Unlimited Cell Growth Model=== | ===Unlimited Cell Growth Model=== | ||
====Physiological basis==== | ====Physiological basis==== | ||
- | Since | + | Since L-forms do not have the cell wall, the shape of the cell is determined by the laws of Newtonian physics and therefore will be as close to the shape of a sphere as possible. For the purposes of this model we will assume that the cell is spherical to start with and therefore will expand evenly in all directions. L-forms of ''Bacillus subtilis'' made with our BioBrick will have an induced mutation in the ''IspA'' gene, which allows the cell to constitutively produce cell membrane phospholipids and therefore the surface area of the membrane will increase over time as the cell grows. Provided that the cell has a sufficient nutrient supply, phospholipids will be produced at a constant rate ''p'', and transported to the surface of the membrane at rate T. Once at the surface, they are inserted into the membrane at rate ''i'', which is determined by the maximum velocity of an enzyme x. These processes will result in an increase of the sphere’s radius at a rate <html><img src="http://latex.codecogs.com/gif.latex?\frac&space;{dr}{dt}&space;=&space;f(r,t,i,p)" title="\frac {dr}{dt} = f(r,t,i,p)" /></html>. In the paper written by [https://2013.igem.org/Team:Newcastle/Modelling/CellShapeModel#References D. Fanelli and A.J. McKane] on "Thermodynamics of vesicle growth and instability" it is explained that the growth of a vesicle is quasistatic in nature, so an equation for growth of the area is given: |
- | + | ||
+ | <html> | ||
+ | <img src="http://latex.codecogs.com/gif.latex?\frac&space;{dA}{dt}=\lambda&space;A&space;\Rightarrow&space;A(t)&space;=&space;A(0)e^{\lambda&space;t}" title="\frac {dA}{dt}=\lambda A \Rightarrow A(t) = A(0)e^{\lambda t}" /></html> | ||
- | However, this model seems physiologically unrealistic. As to allow for the exponential growth of the radius, the cell would have to produce lipids at an exponentially increasing rate, which is larger than the rate of increase of the radius by a factor of 2π. This seems highly | + | However, this model seems physiologically unrealistic. As to allow for the exponential growth of the radius, the cell would have to produce lipids at an exponentially increasing rate, which is larger than the rate of increase of the radius by a factor of 2π. This seems highly improbable, as even at infinite concentration of source lipids inside the cell, the rate at which they are converted to phospholipids and transported to the membrane must be limited by the rate of diffusion, concentration of enzymes, and their turnover rate. While the rate of diffusion and the turnover rate of the enzyme are measurable constants, enzyme concentration is expected to be more or less constant to support homeostasis. |
Therefore we propose a simplistic model of growth which is based on following assumptions: | Therefore we propose a simplistic model of growth which is based on following assumptions: | ||
* the cell is a perfect sphere | * the cell is a perfect sphere | ||
- | * lipids from which the membrane is made are uniformly distributed throughout the cell and the membrane has a constant thickness | + | * lipids from which the membrane is made of are uniformly distributed throughout the cell and the membrane has a constant thickness |
* the cell is in a growth phase throughout the experiment | * the cell is in a growth phase throughout the experiment | ||
* rate of conversion into membrane phospholipids is constant | * rate of conversion into membrane phospholipids is constant | ||
* the insertion of the synthesised membrane lipids is constant and spontaneous | * the insertion of the synthesised membrane lipids is constant and spontaneous | ||
* pressure inside and outside of the cell is quasistatic. | * pressure inside and outside of the cell is quasistatic. | ||
- | * there's | + | * there's sufficient nutrient supply to sustain growth |
===Limitation of Growth by a Set Boundary=== | ===Limitation of Growth by a Set Boundary=== | ||
- | As the maximum volume of the | + | As the maximum volume of the L-forms cell before it divides is unknown, for the purposes of this modelling exercise we assume it's larger than the volume of the chamber and is negligible. Here we work under assumption that the cell grows uniformly in all directions as there's no evidence in the papers that would suggest otherwise. The cell membrane would not adhere to the sides of the chamber, therefore the new membrane would be redistributed towards the spare space, gradually filling the whole chamber. We used a square shape in our model. |
- | |||
- | + | ===Methods=== | |
- | + | Given that a cell is a sphere with a volume <html><img src="http://latex.codecogs.com/gif.latex?V(t)" title="V(t)" /></html> which grows over time as <html><img src="http://latex.codecogs.com/gif.latex?\frac{4}{3}&space;\pi&space;r^3(t)" title="\frac{4}{3} \pi r^3(t)" /></html>, it has a surface area which is dependant on time <html><img src="http://latex.codecogs.com/gif.latex?\inline&space;A(t)=4\pi&space;r^{2}" title="A(t)=4\Pi r^{2}" /></html>. | |
+ | Membrane precursor lipids are being constantly synthesised, and their total mass is equal to <html><img src="http://latex.codecogs.com/gif.latex?\inline&space;M(t)=M_{0}&space;+\kappa&space;t" title="M(t)=M_{0} +\kappa t" /></html>, where <html><img src="http://latex.codecogs.com/gif.latex?\inline&space;M_{0}" title="M_{0}" /></a></html> is the initial mass of membrane lipids in the cell and <html><img src="http://latex.codecogs.com/gif.latex?\inline&space;\kappa" title="\kappa" /></html> is a rate constant. Therefore the area of the cell will grow proportionally to the concentration of precursor lipids in the cell, <html><img src="http://latex.codecogs.com/gif.latex?\inline&space;C(t)=\frac{M(t)}{V(t)}" title="C(t)=\frac{M(t)}{V(t)}" /></html> and a rate constant λ. | ||
- | === | + | Hence, <html><img src="http://latex.codecogs.com/gif.latex?\frac{dA}{dt}&space;=&space;\frac{d4\pi&space;r^2}{dt}&space;=&space;8\pi&space;r&space;\frac{dr}{dt}" title="\frac{dA}{dt} = \frac{d4\pi r^2}{dt} = 8\pi r \frac{dr}{dt}" /></html>, so |
+ | <html><img src="http://latex.codecogs.com/gif.latex?8\pi&space;r&space;\frac{dr}{dt}&space;=&space;\lambda&space;\frac{M}{\frac{4}{3}\pi&space;r^3}" title="8\pi r \frac{dr}{dt} = \lambda \frac{M}{\frac{4}{3}\pi r^3}" /></html>, or | ||
+ | <html><img src="http://latex.codecogs.com/gif.latex?r^4&space;\frac{dr}{dt}&space;=&space;\alpha&space;M" title="r^4 \frac{dr}{dt} = \alpha M" />, where <html><img src="http://latex.codecogs.com/gif.latex?\alpha&space;=&space;\frac{3&space;\lambda}{32\pi&space;^2}" title="\alpha = \frac{3 \lambda}{32\pi ^2}" /></html> | ||
- | + | This can be solved for r(t): | |
- | + | ||
- | + | <html><img src="http://latex.codecogs.com/gif.latex?\int&space;r^4&space;\frac{dr}{dt}dt&space;=&space;\int&space;\alpha&space;M(t)dt" title="\int r^4 \frac{dr}{dt}dt = \int \alpha M(t)dt" /></html> | |
- | + | ||
- | + | ||
- | + | <html><img src="http://latex.codecogs.com/gif.latex?\frac&space;{1}{5}&space;r^5&space;=&space;\alpha&space;\int&space;M(t)dt&space;=&space;\alpha(M_{o}t&space;+&space;\frac&space;{1}{2}\kappa&space;t^2)&space;+A" title="\frac {1}{5} r^5 = \alpha \int M(t)dt = \alpha(M_{o}t + \frac {1}{2}\kappa t^2) +A" /></html>, where a A is an integration constant, determined by setting <html><img src="http://latex.codecogs.com/gif.latex?t=0,&space;r=r\sub_{0}" title="t=0, r=r\sub_{0}" /></html>, so | |
- | \ | + | <html><img src="http://latex.codecogs.com/gif.latex?\frac&space;{1}{5}&space;r^5&space;=&space;A" title="\frac {1}{5} r^5 = A" /></a></html>, so |
- | \frac{1}{ | + | <html><img src="http://latex.codecogs.com/gif.latex?r(t)&space;=&space;(5\alpha(M_{0}t&space;+&space;\frac{1}{2}\kappa&space;t^2)&space;+r_{0}^5)^&space;{\frac{1}{5}}" title="r(t) = (5\alpha(M_{0}t + \frac{1}{2}\kappa t^2) +r_{0}^5)^ {\frac{1}{5}}" /></html> |
- | + | ==Model== | |
- | + | The software of choice for this particular model was MATLAB as it allows a quick visualisation, graphing and mathematical operations. | |
+ | The model was first constructed on paper, then adapted for MATLAB. | ||
- | + | The meaning of each line is explained in green comments. | |
+ | Some of the parameters used in this model were taken from the NCBI database, whereas others were estimated due to lack of information. Initial mass of membrane lipid was predicted to be relative to the general bacterial [http://www.sciencedirect.com/science/article/pii/002228367090255X weight/size]. The rate of lipid synthesis and their conversion into membrane are identical as the integration is known to happen spontaneously. | ||
- | + | <html> | |
- | + | <script type="text/javascript"> | |
+ | SyntaxHighlighter.all(); | ||
+ | </script> | ||
+ | </html> | ||
<pre class="brush: matlab"> | <pre class="brush: matlab"> | ||
Line 72: | Line 76: | ||
cellv=10^(-15); %mean cell volume | cellv=10^(-15); %mean cell volume | ||
- | t_end=70; %growth time | + | t_end=70; %growth time (amount time for which the system is run, and does not equal time during which the cell fills the shape, this time is much smaller and can be determined from the model) |
m=100; | m=100; | ||
lambda=10^(-10); % rate of conversion of mass into area | lambda=10^(-10); % rate of conversion of mass into area | ||
Line 136: | Line 140: | ||
</pre> | </pre> | ||
+ | ===Discussion=== | ||
- | ==Simulation== | + | This model can be improved by conducting experiments which would allow us to find accurate parameters such as the rate of membrane synthesis and maximum membrane torsion. Freeing the model of a few assumptions would also be beneficial. For example if the effects of nutrient depletion were found, and if the maximum size the cell could grow to before dividing was derived, then these could be worked into the model. The model could also be expanded in terms of factoring in the bending energy of the membrane in a particular shape. This would allow us to compare the models of the cells adopting different shapes and to evaluate which shape would me more readily assumed. It would also be interesting to see whether the state of the cell (i.e. L- or rod form) before it enters the chamber has any bearing on the way it fills the space. Also, according to Svatina and Zeks([https://2013.igem.org/Team:Newcastle/Modelling/CellShapeModel#References 2002]), different ratios between the surface area of the membrane and the cell volume yield different cell shapes due to the energy balance involved. We believe that this too may have implications on the cell's behaviour, which can be factored in in the future. |
+ | |||
+ | ===Simulation=== | ||
+ | 2D simulation of the Cell Growth model. | ||
<html> | <html> | ||
- | < | + | <style type="text/css"> |
- | + | #video { | |
- | </ | + | margin-left: 50px; |
+ | } | ||
+ | </style> | ||
+ | <div id="video"> | ||
+ | <video src="https://static.igem.org/mediawiki/2013/8/86/Screen_Recording_3.mp4" width="640" height="360" controls preload></video> | ||
+ | </div> | ||
</html> | </html> | ||
+ | |||
+ | ==References== | ||
+ | |||
+ | [http://www.ncbi.nlm.nih.gov/pubmed/16012516 Cabeen, M.T. and Jacobs-Wagner, C. 2005 Bacterial cell shape. Nat Rev Microbiol. 3:601-10] | ||
+ | |||
+ | [http://www.theory.physics.manchester.ac.uk/~ajm/fm08.pdf Fanelli D., McKane A.J. 2008. Thermodynamics of vesicle growth and instability. Physical Review E 78, 051406] | ||
+ | |||
+ | [http://www.ncbi.nlm.nih.gov/pubmed/12382320 Svetina S., Zeks B. 2002. Shape Behaviour of Lipid Vesicles as the Basis of Some Cellular Processes. The Anatomical Record 268:215-225] | ||
+ | |||
+ | [http://www.ncbi.nlm.nih.gov/pubmed/16959967 Shih Y.L., Rothfield L. 2006. The Bacterial Cytoskeleton. Microbiology and Molecular Biology Reviews p.729-754.] | ||
+ | |||
+ | [http://www.sciencedirect.com/science/article/pii/002228367090255X Mindich L, 1970 Membrane Syntheis in ''Bacillus subtilis'' Journal of Molecular Biology] | ||
+ | |||
{{Team:Newcastle/Sponsors}} | {{Team:Newcastle/Sponsors}} |
Latest revision as of 18:51, 28 October 2013
Contents |
Cell Shape Model
Background
One of our research themes focuses on the ability of L-form bacteria to fit the mould and/or fill spaces by growing into them. We would like to explore the biophysical properties of the cell and the limits of the cell size the L-form can grow to before dividing by constructing a 2-dimensional cell model.
The shape of the bacterial cell is usually determined by the structures of the cell wall and bacterial cytoskeleton. The cell wall of B.subtilis is a thick layer of peptidoglycan which contains cell-wall proteins, techoic and lipotechoic acids. Peptidoglycan is a rigid structure which helps to protect the cell from osmotic pressure and mechanical damage. It also helps the cell to maintain a constant shape, while not specifically defining it. This role is played by the cytoskeleton. The bacterial cytoskeleton is largely similar to that of eukaryotes. It is comprised of three types of protein structures: FtsZ, MreB and crescentin (only present in certain species) which are homologous to eukaryotic tubulin, actin and intermediate filaments respectively. These proteins also perform other functions in the cell; usually they are involved in cell growth and division and therefore are often essential for the cell's survival (Shih and Rothfield, 2006). The communication between the two regulatory components is assured by a series of membrane-associated enzymes (penicillin binding proteins)(Cabeen, Jacobs-Wagner, 2005).
Because L-forms lack the peptidoglycan cell wall, cells naturally adopt the most energetically favourable shape (i.e. sphere) regardless of the cytoskeleton structure. With protoplasts (cells with chemically digested cell wall), the growth, variation in shape and division is restricted due to the limited amount of the cell membrane which simply ruptures if the pressure inside the cell increases. The L-forms created with our BioBrick will have a mutation in the MurE gene which causes spontaneous increase in production of the IspA-like gene product which results in increased synthesis of the cell membrane. This stabilises the cell and allows for growth and division.
Approach
For the purposes of the study the complex model of the growing cell inside of the confined space can be broken down to simpler models of the system in three phases. The first phase would be a constantly growing cell, followed by a model of the cell when it touches the boundaries and therefore changes the trajectory of the membrane growth and finally starts adopting the shape of the boundaries.
Unlimited Cell Growth Model
Physiological basis
Since L-forms do not have the cell wall, the shape of the cell is determined by the laws of Newtonian physics and therefore will be as close to the shape of a sphere as possible. For the purposes of this model we will assume that the cell is spherical to start with and therefore will expand evenly in all directions. L-forms of Bacillus subtilis made with our BioBrick will have an induced mutation in the IspA gene, which allows the cell to constitutively produce cell membrane phospholipids and therefore the surface area of the membrane will increase over time as the cell grows. Provided that the cell has a sufficient nutrient supply, phospholipids will be produced at a constant rate p, and transported to the surface of the membrane at rate T. Once at the surface, they are inserted into the membrane at rate i, which is determined by the maximum velocity of an enzyme x. These processes will result in an increase of the sphere’s radius at a rate . In the paper written by D. Fanelli and A.J. McKane on "Thermodynamics of vesicle growth and instability" it is explained that the growth of a vesicle is quasistatic in nature, so an equation for growth of the area is given:
However, this model seems physiologically unrealistic. As to allow for the exponential growth of the radius, the cell would have to produce lipids at an exponentially increasing rate, which is larger than the rate of increase of the radius by a factor of 2π. This seems highly improbable, as even at infinite concentration of source lipids inside the cell, the rate at which they are converted to phospholipids and transported to the membrane must be limited by the rate of diffusion, concentration of enzymes, and their turnover rate. While the rate of diffusion and the turnover rate of the enzyme are measurable constants, enzyme concentration is expected to be more or less constant to support homeostasis.
Therefore we propose a simplistic model of growth which is based on following assumptions:
- the cell is a perfect sphere
- lipids from which the membrane is made of are uniformly distributed throughout the cell and the membrane has a constant thickness
- the cell is in a growth phase throughout the experiment
- rate of conversion into membrane phospholipids is constant
- the insertion of the synthesised membrane lipids is constant and spontaneous
- pressure inside and outside of the cell is quasistatic.
- there's sufficient nutrient supply to sustain growth
Limitation of Growth by a Set Boundary
As the maximum volume of the L-forms cell before it divides is unknown, for the purposes of this modelling exercise we assume it's larger than the volume of the chamber and is negligible. Here we work under assumption that the cell grows uniformly in all directions as there's no evidence in the papers that would suggest otherwise. The cell membrane would not adhere to the sides of the chamber, therefore the new membrane would be redistributed towards the spare space, gradually filling the whole chamber. We used a square shape in our model.
Methods
Given that a cell is a sphere with a volume which grows over time as , it has a surface area which is dependant on time . Membrane precursor lipids are being constantly synthesised, and their total mass is equal to , where is the initial mass of membrane lipids in the cell and is a rate constant. Therefore the area of the cell will grow proportionally to the concentration of precursor lipids in the cell, and a rate constant λ.
Hence, , so , or , where
This can be solved for r(t):
, where a A is an integration constant, determined by setting , so
, so
Model
The software of choice for this particular model was MATLAB as it allows a quick visualisation, graphing and mathematical operations. The model was first constructed on paper, then adapted for MATLAB.
The meaning of each line is explained in green comments. Some of the parameters used in this model were taken from the NCBI database, whereas others were estimated due to lack of information. Initial mass of membrane lipid was predicted to be relative to the general bacterial [http://www.sciencedirect.com/science/article/pii/002228367090255X weight/size]. The rate of lipid synthesis and their conversion into membrane are identical as the integration is known to happen spontaneously.
%plots a time dependent circle with a growing radius which stops growing cellv=10^(-15); %mean cell volume t_end=70; %growth time (amount time for which the system is run, and does not equal time during which the cell fills the shape, this time is much smaller and can be determined from the model) m=100; lambda=10^(-10); % rate of conversion of mass into area M0=10^(-17); % initial mass of membrane lipids K=10^(-10); %rate of production of the membrane lipids a=10^(-4); %length of the side of a chamber n=100; tspan = linspace(0,t_end,m); r0=(cellv/pi*3/4)^(1/3); %radius of the cell alpha=(3*lambda)/(32*pi^2); % constant which defines the rate at which the radius of the cell grows x=zeros(n); y=zeros(n); x=linspace(-a,+a,n); y=linspace(-a,+a,n); figure(1) clf axis([-a +a -a +a]) hold on r=r0; k=0; while r<=a %below is the code to draw a series of circles representing the cell with a growing radius over the timespan until the cell touches the boundary k=k+1; t=tspan(k); r=(5*alpha*(M0*t+0.5*K*t^2)+r0^5)^(1/5); %radius which changes with time c(k)= 2*pi*r; %circumference of the cell rectangle('Position',[-r,-r,r*2,2r], 'Curvature',[1], 'Edgecolor',[0,0,1], Facecolour, [0,0,1]) %plots the circle with the new radius pause(0.5) radius(k)=r; end; hold all l=0; circ=c(k); crv=1 %curvature (represented by the fracture of the rectangle's side which is curved while crv>0.15 %limit of curvature % the bit below codes for a cycle which draws the new cell outline k=k+1; t=tspan(k); r=(5*alpha*(M0*t+0.5*K*t^2)+r0^5)^(1/5); cn(k)= 2*pi*r; %new cell circumference l=((cn(k)-circ/4); %expansion of the line of coherence between the cell membrane and the chamber crv=1-2*l/a; rectangle('Position',[-a,-a,a*2,2a], 'Curvature',[crv], 'Edgecolor',[0,0,1], Facecolour, [0,0,1]) %plots a rectangle with the side equal to the side of the chamber and curvature determined by the growth of the cell's circumference due to lipid synthesis and integration of lipids into the cell membrane. pause(0.5) radius(k)=r; end;
Discussion
This model can be improved by conducting experiments which would allow us to find accurate parameters such as the rate of membrane synthesis and maximum membrane torsion. Freeing the model of a few assumptions would also be beneficial. For example if the effects of nutrient depletion were found, and if the maximum size the cell could grow to before dividing was derived, then these could be worked into the model. The model could also be expanded in terms of factoring in the bending energy of the membrane in a particular shape. This would allow us to compare the models of the cells adopting different shapes and to evaluate which shape would me more readily assumed. It would also be interesting to see whether the state of the cell (i.e. L- or rod form) before it enters the chamber has any bearing on the way it fills the space. Also, according to Svatina and Zeks(2002), different ratios between the surface area of the membrane and the cell volume yield different cell shapes due to the energy balance involved. We believe that this too may have implications on the cell's behaviour, which can be factored in in the future.
Simulation
2D simulation of the Cell Growth model.
References
[http://www.ncbi.nlm.nih.gov/pubmed/16012516 Cabeen, M.T. and Jacobs-Wagner, C. 2005 Bacterial cell shape. Nat Rev Microbiol. 3:601-10]
[http://www.theory.physics.manchester.ac.uk/~ajm/fm08.pdf Fanelli D., McKane A.J. 2008. Thermodynamics of vesicle growth and instability. Physical Review E 78, 051406]
[http://www.ncbi.nlm.nih.gov/pubmed/12382320 Svetina S., Zeks B. 2002. Shape Behaviour of Lipid Vesicles as the Basis of Some Cellular Processes. The Anatomical Record 268:215-225]
[http://www.ncbi.nlm.nih.gov/pubmed/16959967 Shih Y.L., Rothfield L. 2006. The Bacterial Cytoskeleton. Microbiology and Molecular Biology Reviews p.729-754.]
[http://www.sciencedirect.com/science/article/pii/002228367090255X Mindich L, 1970 Membrane Syntheis in Bacillus subtilis Journal of Molecular Biology]