# Effects of macromolecular crowding on intracellular diffusion from a single particle perspective

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DOI: 10.1007/s12551-010-0029-0

- Cite this article as:
- Hall, D. & Hoshino, M. Biophys Rev (2010) 2: 39. doi:10.1007/s12551-010-0029-0

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## Abstract

Compared to biochemical reactions taking place in relatively well-defined aqueous solutions in vitro, the corresponding reactions happening in vivo occur in extremely complex environments containing only 60–70% water by volume, with the remainder consisting of an undefined array of bio-molecules. In a biological setting, such extremely complex and volume-occupied solution environments are termed ‘crowded’. Through a range of intermolecular forces and pseudo-forces, this complex background environment may cause biochemical reactions to behave differently to their in vitro counterparts. In this review, we seek to highlight how the complex background environment of the cell can affect the diffusion of substances within it. Engaging the subject from the perspective of a single particle’s motion, we place the focus of our review on two areas: (1) experimental procedures for conducting single particle tracking experiments within cells along with methods for extracting information from these experiments; (2) theoretical factors affecting the translational diffusion of single molecules within crowded two-dimensional membrane and three-dimensional solution environments. We conclude by discussing a number of recent publications relating to intracellular diffusion in light of the reviewed material.

### Keywords

‘Crowded’ solutions Brownian motion Single particle intracellular diffusion In vitro reactions Bio-molecules## Introduction

^{1}has reached a high level of predictive capability primarily due to the ability to test and refine the theory using relatively well-defined experimental systems (Doi and Edwards 1999; Batchelor 2000; Byron Bird et al. 2002). In contrast, a predictive theory of diffusion in cell biology has yet to be attained due to the general lack of system definition associated with the type of reaction vessels, i.e. there are many different cell types, with each cell’s internal composition capable of dramatic variation over the very small spatial and temporal scales associated with diffusive motion. Indeed, as indicated by Fig. 1, we are often largely ignorant of the exact chemical surroundings in which our diffusing probe is moving, making the application of complex theory problematic. As a result, our measurements become largely phenomenological in nature and lack ready transferability to other situations. Deciphering observations of diffusive motion made in the complex patchwork collection of microstructures within the cell requires that the discussion of diffusion be conducted within a reductionist framework. In such an approach, general physical principles espoused from the consideration of more highly resolved situations are used to help interpret observations made from small regions of the intracellular molecular landscape (Baumeister 2004). It is towards this viewpoint that we have tailored this review. In the belief that the next step towards a quantitative accounting of intracellular diffusion will be assisted by benchmark conceptualizations of the process, we have reviewed some of the general physical features associated with diffusion in crowded solutions from the perspective of a single molecule’s Brownian motion, giving a simple introduction to the factors responsible for the phenomenon and highlighting methods capable of extracting maximum information from the data. The subject of diffusion is a perennial favourite for review, with many excellent examples on different aspects of the topic (Berg 1993; Saxton and Jacobson 1997; Peskir 2003; Frey and Kroy 2005; Philibert 2006; Dix and Verkman 2008; Saxton 2008). Aware of this fact, we have tried our best to approach the subject matter in a manner that will hopefully prove useful as both a practical and conceptual aid for those actually engaging with the complexities of diffusion in the cell using single particle tracking methods as their experimental avatar.

## Some diffusion basics

^{2}For a large number of particles initially located near to the same region in space, such Brownian motion has the consequence that the particles will tend to disperse over time, this situation being known as diffusion (Fig. 2). At the macroscopic level, the dispersal of the concentration profile of an arbitrary ideal solute component i, C

_{i}(

**r**,t), can be described by Fick’s second law of diffusion

^{3}(Eq. 1a), which is an equation relating the partial time derivative of the concentration to its second partial spatial derivative using a phenomenological

^{4}coefficient of diffusion, D

_{i}(units of m

^{2}s

^{-1}). At the time of its development, the diffusion coefficient was interpreted as a simple constant denoting a shared characteristic of the diffusing component i and the operative solution conditions under which the experiment was conducted. Throughout the period from 1905 to 1908, three scientists, Einstein (Einstein 1956), Smoluchowski (Fulinski 1998) and Langevin (Langevin 1908), all using different approaches, were able to provide a theoretical link between the phenomenological diffusion coefficient utilized by Fick and the system properties governing the individual particle displacements, ∆

**r**

_{i}

**= [**∆x, ∆y, ∆z

**]**

^{T}, occurring over time intervals, ∆t, first observed by Brown (Eq. 1b)

^{5}(Fig. 2).

In this description, k is Boltzmann’s constant, T is the absolute temperature, f_{i} is the particle’s frictional constant, and d is the dimensionality of the Cartesian space involved in the diffusion process. These theoretical predictions relating the diffusion coefficient to the sampling observation time and the particle mean squared displacement (MSD) were confirmed experimentally in the following years by optical microscopy-based observations of colloidal behaviour made by Perrin and co-workers (Perrin 1910) and sedimentation dispersion profiles measured by Svedberg and colleagues in the newly invented analytical ultracentrifuge (Svedberg and Pederson 1940). Importantly, both the theoretical assumptions used to derive Eqs. 1a and 1b as well as the experimental requirements necessary for achieving agreement with the theory, require that the solute particles be dilute and non-interacting—situations which are far removed from the reality inside the cell.

## Experimental measurement of single particle motion within the cell

In correspondence with the macroscopic and particle level descriptions of diffusion embodied by Eqs. 1a and 1b, there are two general approaches for experimental determination of the diffusion coefficient: methods that measure the time-dependent behaviour of a large number (virtual continuum) of particles over relatively large regions of space and methods that involve observing the properties of individual particles over a small region of space. Experimental techniques belonging to the former category include pulsed gradient nuclear magnetic resonance (NMR) (Stejskal and Tanner 1965; Morris and Johnson Jr. 1992; Regan and Kuchel 2003), electron spin resonance (ESR) procedures (Regan and Kuchel 2003; Mirosavljević and Noethig-Laslo 2008), optical microscopy-based observation of light-absorbing or light-emitting solutes (Guo et al. 2008; Lorén et al. 2009), neutron scattering (Doster and Longeville 2007) and single- and multi-wavelength dynamic light scattering experiments (Peetermans et al. 1987). Experimental methods belonging to the later category, i.e. methods capable of observing intracellular single molecule diffusive motion at the microsecond and 100-nm level of precision (approximately) are largely due to technological advances in optical microscopy (Diaspro 2002; Elson 2004; Murcia et al. 2007; Guo et al. 2008). Particular promising from the viewpoint of deciphering the effects of underlying internal cellular structure are the single particle molecule tracking (SPT) techniques (Saxton and Jacobson 1997; Kusumi et al. 2005; Murcia et al. 2007) and the confocal based fluctuation microscopy approaches (Elson 2004; Weiss 2008). As the confocal based fluctuation approaches have been recently reviewed, both in this journal and elsewhere (Elson 2004; Weiss 2008; Chiantia et al. 2009; Jameson et al. 2009), we place our focus in this review on the SPT approach.

**r**(t) (Fig. 3), by repetitive calculation of the position difference vector, ∆

**r**, over an arbitrary time interval, n∆t (Eq. 2).

**D**

_{i}, (Batchelor 2000; Fernandes and de la Torre 2002) may be calculated by sufficiently averaging the successive product of the position difference vector with its transpose, both throughout the trajectory and, where possible, by averaging from multiple particles migrating through the same region of space. (Eq. 3).

^{6}of the system. For isotropic systems, all diagonal elements of

**D**will be equal, and all non-diagonal elements will average to zero, thereby allowing a description of the system by a single diffusion constant D = D

_{xx}= D

_{yy}= D

_{zz}. When this condition is not met, a rotational matrix,

**R**, can be applied to the diffusion tensor with the condition of producing a transformed diffusion tensor

**D′**that is diagonal in nature and necessarily defined in terms of a Cartesian coordinate system x′,y′,z′ that lies along the principle axes of the anisotropy (Eq. 4)

^{(α)}, is shown in Eq. 5 in which the parameter α is termed the anomalous diffusion coefficient.

For normal diffusion, the modifying functional parameter, α, is equal to 1 (Fig. 4c. d). For the case of super-diffusion (D_{i} increasing with time), α is ≥ 1 (Fig. 4e), and in the case of sub-diffusion (D_{i} decreasing with time), α is ≤1 (Fig. 4f). Although the problem is essentially an inverse one, many researchers have used an iterative process of model building and simulation to provide an interpretation of experimentally observed anomalous diffusion in terms of cellular structural characteristics or local solution conditions (Goulian and Simon 2000; Jin and Verkmann 2007; Sanabria et al. 2007; Saxton 2007, Saxton 2008; Weiss 2008). We cite it here as an important descriptor of the diffusion process in crowded solutions (Banks and Fradin 2005; Ridgway et al. 2008; Weiss 2008). It also serves as an important reminder of the importance of asserting the sampling interval time when comparing tracer diffusion coefficients. Indeed, the two limiting forms corresponding to short time n∆t → 0 and long time n∆t →∞ are commonly used for comparative purposes (Bernadó et al. 2004).

## Theoretical description of Brownian motion within the cell

Parallel to the advances in technology that have made high spatial, high temporal frequency single particle tracking a relatively straightforward technique, corresponding developments in computing power have meant that coarse grained particle modelling of cell like situations have started to become a possible, if not routine, addition to the biophysicist’s bag of tools, providing a much required extra level of discrimination in the construction and testing of cellular level biological hypotheses. In general the particle based models available for simulating intracellular diffusion involve the specification of a set number of solute particles within a boundary enclosing volume representing the cell wall (Andrews and Bray 1994; Jeschke 2008; Czech et al. 2009; Moraru et al. 2009; Takahashi et al. 2005; Wils and De Schutter 2009). If one considers the average cell size to be defined by a length scale approximately 10 μm and the average protein radius approximately 2 nm, then it becomes obvious that a full particle representation of the components of the cell is beyond current computing capabilities as it would involve on the order of 1 × 10^{10} particles. To subvert this problem models of intracellular diffusion are ‘coarse grained’ i.e. they are simplified by reducing the number of components and the level of detail. Such modelling approaches often involve simplifications in which Brownian motion characteristics are considered to be independent of the surrounding local environment, and particle interactions (if considered) are incorporated at the level of like/dislike rule based algorithms. Contrarily, much of the higher order theory already developed for the description of diffusion in concentrated solution environments cannot feasibly be employed due to the problems discussed in the introduction relating to general ignorance of the cellular solution composition. In the following section we discuss some of the factors affecting the Brownian motion of single particles in crowded environments and then we review some different levels of approximation for carrying out particle model simulations at different time and length scales commensurate with the level of knowledge of the fine structure of the cell.

### Factors affecting the Brownian motion of single particles in crowded environments

^{th}particle can be calculated as the net force due to the combination of intermolecular potentials acting between explicitly considered particles, (

**F**

_{p})

_{i}, a frictional forces arising from the tendency of the solvent to resist directed motion, (

**F**

_{f})

_{i}, and random forces resulting from unbalanced collisions with the solvent molecules, (

**F**

_{r})

_{i}. When the number of explicitly recognised particles is low the Langevin description approaches its dilute limiting form (Eq. 6a). However at elevated ‘crowded’ conditions the intermolecular potentials become significant and must be accounted for (Eq. 6b).

Although the Langevin equation has limited potential in the simulation of diffusion in crowded systems due to its requirement for short time scales during numerical integration, it provides a very useful pedagogical aid for developing a mechanical understanding of the subject. For now we note that in the concentrated limit the Langevin equation is composed of three force terms, **F**_{p}, **F**_{f} and **F**_{r}, each of which we will discuss in the sections below.

### Forces resulting from intermolecular potentials (**F**_{p})

_{i}and R

_{j}. In general, the intermolecular potentials all feature some form of repulsive interaction at short range that physically arises from electronic repulsion. At longer distances, the interaction may take on attractive or repulsive characteristics empirically defined in terms of a potential energy depth ε and a screening length, L

_{ij}. The potentials described in Fig. 5 and Table 1 are assumed to have spherical symmetry and hence are functions of intermolecular distance, d

_{ij}, only \( \left( {{\hbox{where }}{{\hbox{d}}_{{\rm{ij}} = }}\left| {{{\mathbf{r}}_{\mathbf{i}}} - {{\mathbf{r}}_{\mathbf{j}}}} \right|} \right) \).

Intermolecular potentials commonly used to describe particle interactions and their associated mathematical functions

Pair-potential function | Potential energy function (ΔE | Force derivation [(F |
---|---|---|

Free Overlap | ∆ | ( |

Hard Particle | \( \Delta {E_{ij}} = \left\{ {\begin{array}{*{20}{c}} \infty & {{d_{ij}} < {R_i} + {R_j}} \\0 & {{d_{ij}} \geqslant {R_i} + {R_j}} \\\end{array} } \right. \) | \( \begin{array}{*{20}{c}} {{{\left( {{F_p}} \right)}_i}\,undefined\quad for\quad {d_{ij}}{ < R_i} + {R_j}} \hfill \\{{{\left( {{F_p}} \right)}_i} = 0\,\;for\quad {d_{ij}} > {R_i} + {R_j}} \hfill \\\end{array} \) |

Square Well | \( \Delta {E_{ij}} = \left\{ {\begin{array}{*{20}{c}} \infty & {{d_{ij}} < {R_i} + {R_j}} \\ \varepsilon & {{R_i} + {R_j} \leqslant {d_{ij}} < {R_i} + {R_j} + {L_{ij}}} \\ 0 & {{d_{ij}} \geqslant {R_i} + {R_j} + {L_{ij}}} \\ \end{array} } \right. \) | \( {({F_p})_i} = \left\{ {\begin{array}{*{20}{c}} {undefined} & {{d_{ij}} < {R_i} + {R_j}} \\0 & {{R_i} + {R_j} < {d_{ij}} < {R_i} + {R_j} + {L_{ij}}} \\0 & {{d_{ij}} > {R_i} + {R_j}} + {L_{ij}} \\\end{array} } \right. \) |

Sawtooth | \( \Delta {E_{ij}} = \left\{ {\begin{array}{*{20}{c}} \infty & {{d_{ij}} < {R_i} + {R_j}} \\ {\varepsilon + \left( {\varepsilon /{L_{ij}}} \right){d_{ij}}} & {{R_i} + {R_j} \leqslant {d_{ij}} \leqslant {R_i} + {R_j} + {L_{ij}}} \\ 0 & {{d_{ij}} > {R_i} + {R_j} + {L_{ij}}} \\ \end{array} } \right. \) | \( {\left( {{F_p}} \right)_i} = \left\{ {\begin{array}{*{20}{c}} {undefined} & {{d_{ij}} < {R_i} + {R_j}} \\{\varepsilon /{L_{ij}}} & {{R_i} + {R_j} \leqslant {d_{ij}} < {R_i} + {R_j} + {L_{ij}}} \\0 & {{d_{ij}} \geqslant {R_i} + {R_j}} + {L_{ij}} \\\end{array} } \right. \) |

Soft Sphere | \( \Delta {E_{ij}} = A{\left( {{d_{ij}}} \right)^{ - B}} \) | \( {\left( {{F_p}} \right)_i} = - AB{\left( {{d_{ij}}} \right)^{ - B - 1}}\;for\;all\;{d_{ij}} \) |

Lennard-Jones | \( \Delta {E_{ij}} = 4\varepsilon \left[ {{{\left( {\frac{{{R_i} + {R_j}}}{{{d_{ij}}}}} \right)}^{12}} - {{\left( {\frac{{{R_i} + {R_j}}}{{{d_{ij}}}}} \right)}^6}} \right] \) | \( {\left( {{F_p}} \right)_i} = - 36\varepsilon {\left( {{R_i} + {R_j}} \right)^{12}}{\left( {{d_{ij}}} \right)^{ - 13}} + 24\varepsilon {\left( {{R_i} + {R_j}} \right)^6}{\left( {{d_{ij}}} \right)^{ - 7}} \) |

**F**

_{p})

_{i}, is calculated as the sum of the gradients of the intermolecular potentials existing between the particle under consideration and all of the surrounding explicit species, Eq. 8. The assumption of spherical symmetry requires that the force calculated from each pair potential acts in a direction given by the unit vector \( {\mathbf{\widehat s}} \)acting along the centre-to-centre line between the two particles.

Although the described potential functions and the forces derived from them are not realistic, they serve both heuristic and practical purposes in that they are (1) easy to comprehend, (2) easy to incorporate into simulations and (3) represent an advance to just ignoring these features. Additional features, such as the dependence of the interparticle potentials on such things as ionic strength, can be incorporated phenomenologically by the inclusion of scaling terms in the potential depth and screening length terms (Elimelech et al. 1995).

### Forces resulting from friction exerted by the solvent (**F**_{f})

**v**

_{i}(relative to the velocity of the surrounding fluid), and a frictional constant, f

_{i}, characteristic of the shape of the particle (Dhont 1996; Byron Bird et al. 2002) (Eq. 9a). For spherical particles undergoing translational motion in a 3D solvent environment, f

_{i}is given by Stokes law (Eq. 9b: Jones 2002; Byron Bird et al. 2002). Proteins and lipids in the two dimensions of the cell membrane are usually modelled as upright cylinders (of characteristic radius R

_{i}and cylinder height, H

_{i}) with the frictional coefficient of such a cylinder given by Eq. 9c (Saffman and Delbrűck 1975). In Eqs. 9b and c, η and η′ are the dynamic viscosities (units kg m

^{-1}s

^{-1}) of the solvent or membrane, respectively. Typical values for η and η′ at 37°C are ∼1 × 10

^{-4}and ∼1 × 10

^{-1 }kg m

^{-1 }s

^{-1}, respectively (Byron Bird et al. 2002; Spooner et al. 2000;).

^{7}through a solvent environment must necessarily exert force on the surrounding solvent, which in turn communicates that force to other nearby regions of fluid. This means that the relative velocity between the particle and the surrounding solution environment can no longer be simply equated with the velocity of the particle with respect to an ideal consideration of its local streamline. This additional component to the frictional force, known as the hydrodynamic interaction (HI) force, becomes more pronounced with increasing concentration and level of volume occupation. Consequently, recognition of these HI effects in studies on macromolecular crowding is desirable. Within the Langevin framework, hydrodynamic interactions can be incorporated by including supporting functions containing various degrees of information on the positions, velocities and precise geometries of all N explicitly considered simulation components (Eq. 10a) (Rotne and Prager 1969; Ermak and McCammon 1978; Batchelor 1982; Fernandes and de la Torre 2002; Padding and Louis 2006; Geyer and Winter 2009). As such a precise level of system definition is often lacking when conducting investigations of diffusion within the cell, coarser methods for factoring in HI forces based on effective viscosity have been attempted (Heyes 1995; Wade 1996; Urbina-Villalba et al. 2003; Sun and Weinstein 2007). In this approach, a localized mean field approximation is used to calculate an appropriately averaged scalar value of the frictional coefficient, <

*f*

_{i}>, over the displacement ∆

**r**(Eq. 10b)

*f*

_{i}>, is approximated from the known value of the short-time diffusion constant

^{8}of a tracer particle in a hard particle fluid, with the value either derived from experimental data (Urbina-Villalba et al. 2003) or made using a higher order theoretical method for implementation of hydrodynamic interactions (e.g. Fernandes and de la Torre 2002; Falck et al. 2004; Geyer and Winter 2009). For calculations of tracer diffusion within a solution of identical particles, these averaged values for <f

_{i}> in three dimensions (written in terms of fractional volume ϕ) or two dimensions (written in terms of fractional area θ) are presented as Eqs. 11a and 11b, respectively.

^{9}within a sphere or circle of radius 4R

_{i}centred at position

**r**

_{i}. As an example, Fig. 6 describes the altered frictional force resulting from HI effects experienced by a tracer protein R

_{i}= 2 nm) in an enclosed 2D membrane at either limiting dilution or under crowded conditions (θ = 0.4). The equations derived above should be seen as a first order inclusion of HI as they ignore differences in the perpendicular and parallel components of the viscosity predicted by higher order theory (Elimelech et al. 1995; Dhont 1996; Batchelor 2000).

### Forces resulting from random collisions with the solvent (**F**_{r})

**F**

_{r}(∆t)]

_{i}, written here as a function of the time interval, ∆t, specifying the frequency with which it is updated. A simple conceptualization of the random force term that offers physical insight is that of a thermostat-regulating function (Langevin 1908; Snook 2006) through which it combats the tendency of the viscous frictional force to slow the system down (and hence cool it). The most common procedure for assigning a numerical value to [

**F**

_{r}(∆t)]

_{i}involves requiring that it conforms to relations derived from application of the fluctuation dissipation theorem (Eq. 12) (Kubo 1966).

^{10}the temperature and the local frictional coefficient (Saxton 2008). The mathematics behind the result presented in Eq. 12 can be relatively difficult to follow so here we offer a simple argument which although only yielding an approximate result provides some useful insight into the physical origins of the random force and the natural time constant of the system. In this simplified model, the average kinetic energy of the system is first equated with the average thermal energy via the equipartition theorem, i.e. \( \left\langle {m{v^2}} \right\rangle = d{k_B}T \) therefore, \( v \leqslant \sqrt {{d{k_B}T/m}} \). Over time scales sufficiently small enough to preserve inertial memory, we can equate the average magnitude of the random force with the average absolute value of the frictional force (Eq. 13a), with this relationship being further developed by combination with the relation for the average particle velocity to determine the magnitude of the random force term (Eq. 13b).

_{i}> has units of time and can thus be interpreted as specifying a natural time constant for the system, such that \( \Delta \tau = {\hbox{m}}/ < {{\hbox{f}}_{\rm{i}}} > \). For specification of larger time intervals ∆t >> ∆τ, such a direct physical interpretation of the random force term breaks down due to the fact that the path taken between the application of the intervening stochastic random forces is not linear, but rather occurs as the result of a random walk produced by many collisions, each occurring at or around the natural time constant of the system. In this time regime, the average motion of the particle is best described as a function of its mean squared displacement (Langevin 1908; Einstein 1956) (Eq. 1b). Using that definition of the diffusion coefficient, a phenomenological velocity can be determined over the time step and calculated displacement (Eq. 14)

### Using the Langevin equation to simulate diffusion at different time scales

_{o}= ∆t

^{11}, to yield Eq. 16.

The upper limit for the time step, τ_{B} = ∆t, chosen for numerical integration in the Brownian dynamics regime corresponds to a value which prevents particles from passing through each other over the interval. For systems composed of particles of a single radius R_{i}, τ_{B} ∼ R_{i}^{2} <f_{i}>/(2d k_{B}T). Due to its simplicity and ability to access larger time scales, Eq. 17b is particularly suitable for examining diffusion in crowded solution environments.

_{B}Eq. 17b can be first be used to produce a sufficiently long time simulation to allow for the desired time interval diffusion tensor,

**D**

_{i}(n∆t), to be either directly calculated from the data using the methods shown in Eq. 3 or alternatively estimated by extrapolation. This diffusion tensor can then be used in conjunction with a unit vector \( {\mathbf{\widehat m}} \) to simulate Brownian motion over the homogenous phase using relatively large time steps as a form of the position Langevin simulation method (Lax 1966; Zwanzig 1969; Hall 2008; Hall 2010) (Eq. 18a). In this approach each component in the displacement vector, ∆

**r**

_{i}(n∆t), is randomly chosen from a Gaussian distribution of zero mean and standard deviation given by the component term indicated by Eq. 18b.

## Discussion of recent experimental findings

^{12}indicate that for intermediate crowding regimes, the effect of a repulsive potential is to increase the magnitude of the short-time diffusion coefficient by helping to keep the tracer particle out of the ‘stagnant’ region associated with high local densities of background particles. Not surprisingly, the effect of a weakly attractive potential shows the reverse behaviour, with the tracer diffusion coefficient decreasing due to a combination effect arising from the attractive intermolecular potential (i.e. larger particles diffuse more slowly) and the HI forces (i.e. the tracer spends more time located in higher viscosity regions). The purely hard sphere tracer case with no associated potential was also simulated and is intermediate between the two

^{13}. The time dependence of the diffusion coefficient was also analysed and is displayed in Fig. 7 e, f for the three different types of associated intermolecular potential. All three examples demonstrated anomalous diffusion characteristics (α ≈ 0.85) similar in magnitude to those previously measured (Banks and Fradin 2005; Szymanski and Weiss 2009).

Modelling approaches capable of accounting for such complex diffusive behaviour as that described above are required if we are to develop predictive models of intracellular diffusion. Towards the development of a such a predictive theory explicit accounting for the spatial dimension is an important first step. Methods for factoring in the dimensions of the cellular reaction vessels have been implemented in programs such as MCELL (Czech et al. 2009), VIRTUAL CELL (Moraru et al. 2009), E-CELL (Takahashi et al. 2005) and STEPS (Wils and De Schutter 2009) by incorporation of structures from confocal or EM image traces. However, as we have noted in this review diffusive, transport processes occurring in solution are not just affected by geometric considerations, but also by a combination of intermolecular potentials, hydrodynamic interactions and random forces effected by the solvent. Recent modelling and simulation efforts have started to address some of these issues (Bicout and Field 1996; Andrews and Bray 2004; Takahashi et al. 2005; Jeschke 2008; Czech et al. 2009; Moraru et al. 2009; Wils and De Schutter 2009). It is towards the goal of providing a readily digestible review of the general physical factors affecting Brownian behaviour that we have endeavoured to achieve here.

## Concluding remarks

The general area of study relating to how the complex structured microenvironment of the cell affects the fate of biochemical reactions occurring within it has been termed as ‘macromolecular crowding and confinement’ or simply ‘crowding’ for short (Minton and Wilf 1981; Harris and Winzor 1985; Minton 1992; Zhou et. al. 2008). Despite the fascination that ‘biological chemistry’ holds for many, the study of intracellular crowding effects is a difficult subject area in which to both design and conduct experiments and to theoretically interpret the experimental results (Zimmerman and Minton 1993; Hall and Minton 2003; Zhou et al. 2008). In conventional biochemical investigations complications arising from unwanted side-reactions are made tractable via reduction of the number and extent of variable system components (Goto et al 1993; Hoshino et al 1997). However, even in in vitro model system approximations of crowding, such an option is limited when the objective is to examine the effect of a complex and highly concentrated background environment of the biochemical reaction at hand. The situation becomes more difficult when studying crowding in, in vivo, model systems due to a lack of definition/knowledge of both the composition (Zimmerman and Trach 1993; Ma'ayan et al. 2005) and position (Luby-Phelps et al. 1988; Diaspro 2002; Leis et al. 2009) of the system components. Often times, the irreducible nature of the experimental system can lead to the presence of multiple competing effects which can confound the ready application of theoretical methods. As such, the ability of modelling approaches for generating easily accessible guiding principles has generally been inversely proportional to their degree of realism (Zimmerman and Minton 1993; Schnell and Turner 2004; Sear 2005; Hall and Dobson 2006; McGuffee and Elcock 2006; Qin and Zhou 2009). Relatively simple models of diffusion in crowded solution have provided considerable insight into diffusive behaviour within cells (Muramatsu and Minton 1988; Minton 1989; Han and Herzfeld 1993; Hall 2008, Hall 2010). Recent advances in both single particle tracking (Saxton and Jacobson 1997, Kusumi et al. 2005; Murcia et al. 2007; Hellriegel and Gratton 2009) and single particle simulation methods (Bernadó et al. 2004; Sun and Weinstein 2007; Dix and Verkman 2008; Ridgway et. al. 2008; Weiss 2008) hold the promise that as we move into the new decade our potential to understand diffusive behaviour within the complex confines of the cell will continue to grow – perhaps putting a predictive theory of diffusion within the cell within eventual reach.

This review is restricted to the discussion of diffusion in low Reynolds number fluid systems (the Reynolds number is a dimensionless parameter reflecting the relative importance of inertial to viscous forces), which are good approximations of the intracellular environment.

After the botanist, Robert Brown, who first noted it while observing pollen grains under a microscope in the early 1800s.

Adolf Fick published a series of papers on diffusion in 1855 (a modern analysis of his observations of the diffusion of salt is provided by Philibert 2006). By likening the diffusion of ions in solution to the flow of heat, Fick was able to adopt the mathematical methods developed by Fourier, thus explaining why the diffusion equation is near identical to equations developed for modelling heat flow.

Einstein was first, closely followed by Smoluchowski second; therefore, the relationship is alternately called the Einstein relation or the Einstein–Smoluchowski equation.

Isotropy refers to the equivalence of a given process along different directions through the medium.

In this instance directed motion refers to the short steps with transient direction associated with Brownian motion.

The value of q = 1 at time scales small enough (∆t < m/<f_{i}>) to preserve inertial memory, whereas q = 2 for time scales greater than this ((∆t > m/<f_{i}>).

Note this integration is based on the assumption that all force terms are constant over the time interval, ∆t, for which the integration is carried out. Additionally we have introduced a factor q here to describe the different time interval ranges i.e. when ∆t < ∆τ, q = 1 and when ∆t >> ∆τ, q = 2d.

The predicted reduction in diffusion coefficient for the hard cylinder and sphere cases shown in Fig. 7 is slightly steeper than suggested by previous theoretical results for unbounded systems (3D: Tokuyama and Oppenheim, 1994; 2D: Bussell et al. 1995 superimposed in green), with the discrepancy due to our simulations being performed in a repulsive cylindrical/spherical container not featuring periodic boundary conditions.

## Acknowledgements

We would like to acknowledge Prof. M. Okuwaki, Prof. D. Stanley, Dr. N. Hirota and Dr. M. Nemoto for providing helpful comments on an early draft of this manuscript. We also greatly appreciate the insightful reviews provided by Dr. Allen P. Minton and the anonymous reviewer 2 which helped to significantly improve the paper. This research was supported by grants to D.H. from the Japanese Science and Technology Agency (JST) and the University of Tsukuba under the special coordinated scheme ‘Funds in Aid for the Promotion of Young Scientists’ Independent Research’ and to M.H. from ‘Grants-in-Aid from the Japanese Ministry of Education, Culture, Sports, Science and Technology’.