Team:Edinburgh/Cellulases (MATLAB model)

From 2011.igem.org

Cellulases (MATLAB model)

MATLAB is a general-purpose mathematical tool, developed by [http://www.mathworks.com Mathworks], and commonly used by engineers. Among other things, it can be used to solve ordinary differential equations (ODEs) by numerical integration.

An attempt was made to use MATLAB to model the degradation of cellulose into glucose in a biorefinery. But accurately predicting how much is converted in the synergistic system (where enzymes are kept close together) is difficult without literature to provide the ODEs and the kinetic parameters. Therefore this model only looks at the free floating (non-synergistic) enzyme approach. It is deterministic and is set by a series of initial conditions.

Contents

Assumptions

The mathematical model is based on the ODEs and kinetic parameters outlined in [http://onlinelibrary.wiley.com/doi/10.1021/bp034316x/full Kadam et al (2004)]. The following are its assumptions and basis:

  • Underlying assumption: cellulose, cellobiose, and glucose concentrations change continuously with time.
  • Rate equations assume enzyme adsorption follows the Langmuir isotherm model.
  • Glucose and cellobiose, which are the products of cellulose hydrolysis, are assumed to "competitively inhibit enzyme hydrolysis".
  • All reactions are assumed to follow the same temperature dependency Arrhenius relationship (shown below). However, in reality it should be different for every enzyme component, "because of their varying degrees of thermostability, with β-glucocidase being the most thermostable. Hence the assumption is a simplification of reality".
  • Conversion of cellobiose to glucose follows the Michaelis-Menten enzyme kinetic model.

Equations

Rate Equations

Cellulose to cellobiose reaction with competitive glucose, cellobiose and xylose inhibition.
Cellulose to glucose reaction with competitive glucose, cellobiose and xylose inhibition.
Cellobiose to glucose reaction with competitive glucose, cellibiose and xylose inhibition.

Constants

knr — reaction rate constant for reaction n
EnB — the bound concentration for exo and endo-β-1,4-glucanase for reaction n
Rs — substrate reactivity parameter
S — substrate reactivity at a given time (g/kg)  
G2 — concentration of cellobiose
G — concentration of glucose  
X — xylose concentration  
KnIG2 — inhibition constant for cellobiose at reaction n
KnIG — inhibition constant for glucose at reaction n
KnIX — xylose inhibition constant for reaction n

Note: For simplicity's sake we have assumed no xylose in the system, therefore X=0.

Langmuir Isotherm

The Langmuir Isotherm model mathematically describes enzyme adsorption onto solid cellulose substrates. Even though the Langmuir model is based on uniform binding sites and no interaction between the adsorbing molecules, it is not valid for cellulase adsorption onto cellulose. "Nevertheless the Langmuir formulation remains useful for mathematically describing the phenomenon of enzyme adsorption" ([http://onlinelibrary.wiley.com/doi/10.1021/bp034316x/full Kadam et al, 2004]).

Constants

exo and endo-β-1,4-glucanase, i=1  
β-glucosidase, i=2  
Eimax — Maximum mass of enzyme that can be absorbed onto a unit of mass substrate
Kiad — Dissociation constant for enzyme i
EiF — Free enzyme concentration for enzyme i
S — Substrate reactivity at a given time (g/kg)

Mass Balances

Cellulose mass balance
Cellobiose mass balance
Glucose mass balance

Arrhenius Equation

Arrhenius equation is an empirical relationship which is used to model the temperature dependent reaction rate constant. Note: T1 is set at 45 °C

Constants

Kir — Reaction rate constant of reaction i
Eai — Activation energy of reaction i
R — Universal gas constant

Construction of Model

The model was constructed using the numerical programme MATLAB. A script file was generated which holds the variable dictionary, constants, temperature dependency equations, the "ODE45" differential equation solver, and the plot command.

A separate function file to the script is created as script files can only operate on the variables that are coded into their m-files. Rs (the substrate reactivity parameter) changes at every iteration because it is dependent on the S the substrate concentration at a given time, the substrate being cellulose. Therefore S at the first iteration is S0, the initial substrate concentration. At the second iteration S is the previous value calculated by the ODE, and so on. After each step the new value of S is fed into the function file and is used for calculating the reaction rate constant for cellobiose and glucose, etc.

Rs — substrate reactivity equation

ODE45 calls on the function file to calculate the rate equations and then substitute them into the respective mass balance. A numerical integration is performed and the results can be seen below. ODE45 is used as it is more accurate than other solvers [http://www.mathworks.co.uk/help/techdoc/ref/ode23.html (according to Mathworks)]. It is based on an explicit Runge-Kutta formula and is a one-step solver.

Results

Figure 1: Graph of cellulose degradation over time with maximum β-glucosidase.
Initial conditions: Cellulose - 100 g/kg, Glucose - 0.01 g/kg , Cellobiose - 0.01 g/kg.
Enzymes: Exo/endo-glucanase - 0.01 g/kg, β-glucosidase - 1 g/kg
Temperature 35° C


Figure 2: Graph of cellulose degradation over time with maximum Exo/endo-glucanase.
Initial conditions: Cellulose - 100 g/kg, Glucose - 0.01 g/kg , Cellobiose - 0.01 g/kg.
Enzymes: Exo/endo-glucanase - 1 g/kg, β-glucosidase - 0.01 g/kg
Temperature 35° C

Figure 1 is set with β-glucosidase at its maximum concentration and Figure 2 with Exo/endo-glucanase at maximum. This is to compare the effect of certain enzymes on cellulose degradation and glucose production. The result is consistent with what is expected. Exoglucanase chews away at the end of a cellulose chain, producing cellobiose sugars and endoglucanase cuts cellulose chanins in the centre, turning one chain into two. This concurs with the results, with Figure 1 modelling markedly higher amount of cellulose at the minimum amount of exo/endo-glucanase than that of Figure 2. Whereas β-glucosidase cuts cellobiose in half, producing two glucose molecules. Figure 2 which β-glucosidase is at its maximum produces 255.6% more glucose than in Figure 1 with β-glucosidase at its minimum in 60 hours.

The concentration of cellobiose in Figure 1 keeps low. This is because there is little cellulose converted to cellobiose by Exo/endo-glucanase. Also, if there is any cellobiose, they are all converted to glucose by β-glucosidase.

Figure 3: Graph of cellulose degradation over time with maximum β-glucosidase.
Initial conditions: Cellulose - 100 g/kg, Glucose - 0.01 g/kg , Cellobiose - 0.01 g/kg.
Enzymes: Exo/endo-glucanase - 1 g/kg, β-glucosidase - 0.01 g/kg
Temperature 35° C. The x-axis is set to semilog.

Figure 3 is under the same conditions as Figure 2, but its x-axis is set to a semilog scale to illustrate what happens over a longer period of time. The effect of high β-glucosidase can better be seen with the complete conversion of cellobiose to glucose.

(We'd like to thank the ETH Zurich team for submitting some bugfixes to the simulation that led to this figure; where previously it violated the laws of physics, now it does not!)

Download MATLAB file

You can download the ready model as a .zip file:

Download the model file here

References

  • Kadam KL, Rydholm EC, McMillan JD (2004) [http://onlinelibrary.wiley.com/doi/10.1021/bp034316x/full Development and Validation of a Kinetic Model for Enzymatic Saccharification of Lignocellulosic Biomass]. Biotechnology Progress 20(3): 698–705 (doi: 10.1021/bp034316x).