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First published online July 5, 2006
doi: 10.1242/10.1242/jcs.03063
Commentary |
Section on Physical Biochemistry, Laboratory of Biochemical Pharmacology, National Institute of Diabetes and Digestive and Kidney Diseases, National Institutes of Health, US Department of Health and Human Services, Bethesda, MD, USA
e-mail: minton{at}helix.nih.gov
Accepted 23 May 2006
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Summary |
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 Top Summary IntroductionTypes of background and...A common energetic formalismPredictions and observationsRelevance to cell biologyReferences |
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Key words: Protein associations, Protein stability, Protein folding, Macromolecular crowding, Macromolecular confinement, Macromolecular adsorption
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Introduction |
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TopSummaryIntroductionTypes of background and...A common energetic formalismPredictions and observationsRelevance to cell biologyReferences |
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Types of background and background interactions |
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TopSummaryIntroductionTypes of background and...A common energetic formalismPredictions and observationsRelevance to cell biologyReferences |
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). Since no single macromolecular species need be present at high concentration, such media are referred to as crowded or volume occupied rather than concentrated (Minton and Wilf, 1981). Since macromolecules cannot interpenetrate, the fraction of volume into which a macromolecule can be placed at any instant is much less than the fraction of volume into which a small molecule can be placed (Fig. 2A,B). The total free energy of interaction between X and all of the other molecules in the crowded medium is inversely related to the probability of successful placement of X at a random location within the crowded medium (Lebowitz et al., 1965). Hence the extra work required to transfer X from a dilute to a crowded solution resulting from steric repulsion between X and background molecules depends upon the relative sizes and shapes of X and background species, and increases in a highly nonlinear fashion with increasing size of X and with fractional volume occupancy (Minton, 1998).
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). It has been estimated that between 10% and 100% of the fluid phase of the cytoplasm lies within one macromolecular diameter of the surface of one of these structures (Minton, 1989). By analogy with size exclusion columns, we may generically treat these interstitial elements of fluid volume as `pores'. When the size of a pore is not much larger than that of an enclosed macromolecule reactant X, steric-repulsive interactions between X and the pore boundaries result in a reduction of the volume available to X (Fig. 2C,D). Hence work (free energy) is required to transfer a molecule of X from an element of unbounded solution into a pore of equal volume (Giddings et al., 1968). The magnitude of excess work depends strongly upon the relative sizes and shapes of both the confined macromolecule and the pore (Giddings et al., 1968; Minton, 1992).
Macromolecular adsorption
When X bears a net charge opposite to that of the surface of a nearby fiber or membrane, X may be reversibly nonspecifically adsorbed onto the surface (Cutsforth et al., 1989; Knull and Walsh, 1992; Lakatos and Minton, 1991). Similarly, if X is a post-translationally modified protein bearing a lipid side chain, it may also reversibly and nonspecifically adsorb onto lipid bilayer membranes (Arbuzova et al., 1998). When surface adsorption is spontaneous, the associated free energy change is negative, but its magnitude depends on entropic factors that vary nonspecifically with the size and shape of X (Minton, 1995).
Influence of background interactions upon reaction equilibria and rates
Fig. 3 illustrates how nonspecific interactions between reactants and the background can influence the rate and/or equilibrium of a particular reaction – for example the association of two globular proteins, A and B, to form a heterodimer. In this reaction, the `reactants' are A and B separated by a distance sufficiently large that they do not interact, and the `product' is the heterodimer. In the `transition state', A and B are close to each other and orientated such that they are poised to form the heterodimer, but they are still not bound to each other by short-range attractive interactions.
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500 g/l in some compartments) that the sum of a large number of weak, nonspecific interactions can contribute substantially to the standard free energy of each state of the reaction system. The free energy profile in green in Fig. 3 has been shifted downwards because all three states of the system interact with the background in an attractive (free energy lowering) fashion. Such nonspecific intermolecular attraction can be due to weak electrostatic or hydrophobic effects and often results in the formation of weak, nonspecific complexes (e.g. the interaction of proteins with urea). The important feature of this profile is that the relative free energies of the three states of the system have also been altered: the background interactions stabilize the transition state and products more than they do the reactants. These background interactions should therefore push the equilibrium state towards product formation, primarily by enhancing the forward reaction rate.
By contrast, the free energy profile in red in Fig. 3 has been shifted upward because all three states of the system interact with the background in a repulsive (free energy raising) fashion. Nonspecific intermolecular repulsion can be due to volume exclusion (steric repulsion) or electrostatic effects and does not lead to formation of complexes between the mutually repelling species. Nevertheless, because the repulsive interactions in this example destabilize the reactant state more than they do the transition and product states, the overall effect upon the relative free energies of the three states is identical to that above. The equilibrium is shifted towards product formation, because of a preferential increase in the forward reaction rate. Note that even though the mechanisms underlying these two perturbations of the free energy profile are different, one cannot distinguish between them solely by measuring changes in reaction equilibria or kinetics.
There are many other combinations of repulsive and attractive background interactions that can lead to the same relative shifts in the free energies of the three reaction states and hence the same changes in reaction rates and equilibria. By considering the molecular composition and environmental variables characterizing a particular reaction system, one may discern whether dominant background interactions are likely to be attractive or repulsive. But in a medium as complex and heterogeneous as the cytoplasm for example, the task of identifying these and their influence on any specific reaction is extremely challenging.
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A common energetic formalism |
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TopSummaryIntroductionTypes of background and...A common energetic formalismPredictions and observationsRelevance to cell biologyReferences |
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cAB/cAcB, is related to the standard free energy of association, 
FAB, by the thermodynamic relationship:
 | (1) |
. We may construct thermodynamic cycles that relate the free energies of association in the absence and presence of background interactions (Fig. 5), because free energy is conserved around the cycle:
 | (2) |
denotes the standard free energy of association of A and B in the absence of background interaction and FI,X denotes the standard free energy of interaction between X and the background. It follows from equations 1 and 2 that:
 | (3) |
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FI,X is positive or negative (see Fig. 3).
Note that, although equations 1-3 are entirely general, each type of background interaction results in a distinctly different dependence of FI,X upon the size and shape of X and the sizes, shapes and fractional volume occupancies of those background constituents with which X interacts.
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Predictions and observations |
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TopSummaryIntroductionTypes of background and...A common energetic formalismPredictions and observationsRelevance to cell biologyReferences |
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; Minton, 1992; Minton, 1995; Zhou and Dill, 2001; Zhou, 2004). These are based upon mesoscopic or coarse-grained models that take into account the molecular nature of the individual reactant species, but adopt simplified representations of the molecules and the interactions between them. Such models cannot account quantitatively for the behavior of macromolecules in environments as complex and intrinsically variable as the cytoplasm or nucleoplasm. However, they successfully predict large effects of `inert' background substances upon a variety of reaction rates and equilibria in vitro (see Tables 1, 2, 3). In favorable cases, the magnitude of the observed effects agrees quantitatively with theoretical prediction. Data demonstrating the effects of crowding are shown in Fig. 5. Each of the effects was predicted qualitatively by one of the theories cited above.
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Relevance to cell biology |
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TopSummaryIntroductionTypes of background and...A common energetic formalismPredictions and observationsRelevance to cell biologyReferences |
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, but are such effects similarly important in a living cell? On the basis of results obtained from partitioning and size-exclusion experiments conducted with concentrated cell lysates, Zimmerman and Trach estimated that excluded volume effects in the cytoplasm of E. coli are comparable to those obtained in a 35% solution of a 70 kDa globular protein, such as bovine serum albumin or hemoglobin (Zimmerman and Trach, 1991). Although this estimate might provide a useful starting point, it is clear that the answer is far more complex and elusive. Any cell is extremely large relative to any particular macromolecule of interest and is likely to contain several micro-environments, within each of which a particular macromolecule X will be subject to a different set of background interactions. For example, the cytoplasm of even an organism as simple as E. coli contains at least three such micro-environments: the immediate vicinity of the inner plasma membrane, within which X will encounter a high local concentration of membrane phospholipids and proteins; the interior and immediate vicinity of the nucleoid, within which X will encounter an extremely high local concentration of DNA; and the remaining cytoplasm, within which X will be subject primarily to the influence of other soluble proteins. One would expect the relative contributions of macromolecular crowding, confinement and adsorption to macromolecular reactivity to be rather different within each of these three micro-compartments. That complexity acknowledged, it is nevertheless true that large and unambiguous background effects have indeed been observed within certain specialized, simplified cells.
The interior of an erythrocyte is essentially a highly concentrated solution of hemoglobin. The affinity of erythrocytes containing sickle cell hemoglobin (HbS) for oxygen depends significantly upon the intracellular hemoglobin concentration, because oxygen binding is linked to the polymerization of HbS (May and Huehns, 1975). The concentration dependence of oxygen affinity may be quantitatively accounted for if, and only if, steric repulsion between hemoglobin molecules is taken into account (Minton, 1976). Ferrone has recently reviewed a large body of work demonstrating that the extensively characterized kinetics of cell sickling subsequent to deoxygenation may be well accounted for by models that take into account the substantial effect of macromolecular crowding within erythrocytes upon the thermodynamic activity (effective concentration) of monomers and each oligomer in the hemolyzate (Ferrone, 2004). By means of cleverly designed experiments, volume regulatory mechanisms in dog erythrocytes were shown to respond nonspecifically to changes in the intracellular concentration of macromolecules rather than changes in volume per se (Colclasure and Parker, 1992).
The interior of an eye lens cell consists essentially of a solution of a small number of crystallins at very high concentration (total protein concentration >500 g/l). These proteins are not translated postnatally. Thus, the crystallin molecules that an animal is born with must remain structurally intact over much of its lifetime to preserve lens transparency. The thermal stability of these proteins increases with concentration (Steadman et al., 1989), and the extraordinary thermal stability of an intact lens has been attributed in part to the stabilizing effects of macromolecular crowding inside the lens cell (Bloemendal et al., 2004).
Excluded volume theory predicts that at the high levels of fractional occupancy characterizing almost all biological fluid media, even small changes in cellular hydration will result in disproportionately large changes in the reactivity of a broad spectrum of macromolecular reactants. This prediction is consistent with and may account for the following general observations: (1) Relatively modest changes of cellular volume in animal cells are associated with changes in a wide variety of diverse intracellular processes, such as the polymerization/depolymerization of cytoskeletal filaments or the activation/deactivation of membrane ion channels, that are much too large to be accounted for on the basis of simple mass action (reviewed by Lang et al., 1998). (2) Complex and very diverse systems for maintaining the concentrations of cellular contents within narrow limits have evolved within all life forms, be they bacterial, plant or animal (Somero et al., 1992). (3) The age-related onset of a variety of protein-aggregation-linked diseases (Koo et al., 1999) correlates with significant loss of cellular and tissue hydration in the elderly and concomitant increases in the volume excluded to protein (Parameswaran et al., 1995; Hatters et al., 2002).
During the last few years several experimental techniques have been developed that enable certain aspects of the behavior of selected macromolecules – typically labeled and/or overexpressed – to be monitored within living cells (e.g. Ghaemmaghami and Oas, 2001; Ignatova and Gierasch, 2004; McNulty et al., 2006). It is hoped that techniques like these, or others yet to be devised, can be used to investigate the influence of background interactions upon the behavior of the selected species within their native environments. However, one must be extremely cautious about interpreting the results of such experiments. In particular, it is necessary to design and carry out control experiments that clearly indicate whether or not the processes of labeling and/or overexpression result in abnormal distribution of the selected protein within the cell, induction of artifactual associations, or disruption of the normal background interactions that one is attempting to investigate.
This Commentary bears as its title the provocative question "How can biochemical reactions within cells differ from those in test tubes?" When one can specify the composition of the local environment of a particular reaction at a specific intracellular location and at a particular time point in the cell cycle, studies such as those cited here will help to provide answers to the equally interesting and perhaps more biological question "By how much do biochemical reactions within cells differ from those in test tubes?"
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Acknowledgments |
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Footnotes |
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Free energy changes denoted by F may refer to either Gibbs or Helmholtz free energies since the relationships described here hold equally in constant pressure and constant volume systems.
Predicted effects of macromolecular confinement on association equilibria have not yet been tested.
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) and presence (
) of 100 g/l Ficoll 70 (del Alamo, 2005). The half-time for assembly of the protein is decreased ten-fold in the presence of Ficoll. (C) Temperature dependence of the ellipticity of 
-lactalbumin in bulk solution (
) and encapsulated in hydrated silica sol-gel glass (
). The confined protein behaves normally at low temperature, but exhibits only partial unfolding even at temperatures approaching 100°C. Figure reproduced with permission from Eggers and Valentine (Eggers and Valentine, 2001