Difference between revisions of "The Science of Mashing"

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==Inhibitors and cofactors==
 
==Inhibitors and cofactors==
  
Some enzymes require the presence of a non protein compound, commonly a metal ion, for the reaction. Without this cofactor the enzyme is not able to catalyze the reaction it was made for. As a result the rate of the enzymatic reaction may also be limited by the concentration and availability of the necessary cofactors. One important cofactor for enzymes needed by the yeast metabolism is for example zink.
+
Some enzymes require the presence of a non protein compound, commonly a metal ion, for the reaction. Without this cofactor the enzyme is not able to catalyze the reaction it was made for. As a result the rate of the enzymatic reaction may also be limited by the concentration and availability of the necessary cofactors. One important cofactor for enzymes needed by the yeast metabolism is for example zink [wikipedia.org]
  
 
Inhibitors reduce the reaction rate of the enzymes.
 
Inhibitors reduce the reaction rate of the enzymes.

Revision as of 04:38, 30 November 2008

------------- Work in progress ------------

In mashing the milled grain (grist) is mixed with water to create the mash. It is an essential process in the production of beer and a continuation of the malting process on the way to sweet wort. During the mash soluble malt compounds like enzymes, proteins and sugars are dissolved by the mash water and insoluble malt compounds like starch and some long chained proteins are converted into soluble compounds and dissolved into the water. The latter happens through a combination of physical and biochemical process which can be controlled by the brewer to achieve a sweet wort of desired quality. The biochemical processes are catalyzed by various malt enzymes. Their function and behavior is dependent on the conditions in the mash (e.g. temperature, pH, concentration, etc.) and the brewer should be familiar with that behavior in order to control the quality of the sweet wort that is run off from the mash in the lautering process.

Enzymes

Figure 1 - A simplified illustration of beta amylase splitting maltotetraose into two maltose molecules. A - a beta amylase molecule bonds to the non reducing end of the glucose chain. Because of its shape it fits only there. B - The intermediary bond reacts with a water molecule. C - The reaction releases 2 maltose molecules and frees the beta amylase molecule

Enzymes are very important to mashing. They catalyze conversion reactions which break down malt compounds (the largest one being starch). In the case of starch this conversion is necessary to form water soluble dextrines and sugars. The latter of which can be metabolized by the yeast. Enzymes are proteins (chains of amino acids) which have the ability to lower the energy needed for a chemical chemical reaction which allows that reaction to occur faster and at lower temperatures. Most enzymes are very specific to the reaction they catalyze and work only with a specific substrate and produce only a specific product. In case of the beta amylase enzyme, for example, the substrate is a glucose chain and the product is maltose. The reaction that is catalyzed the the split of a glucose chain link while a molecule of water is consumed. The highly specific nature to the reaction that is catalyzes stems form the shape of the enzyme which is just right for reacting with the substrate and releasing the product and residual product shortly after. The enzyme itself is not consumed in the reaction. I.e. once free again it can catalyze another reaction.

Without an enzyme a chemical reaction may look like this [rsc.org]:

substrate1 + substrate2 -> product

But the initial energy (i.e. temperature) needed for this reaction may be so high that it rarely ever happens. With the presence of an enzyme this reaction changes to

substrate1 + enzyme -> enzyme-substrate-intermediate
enzyme-substrate-intermediate + substrate2 -> product + enzyme

The energy needed for these enzymatic reactions are now low enough for the reaction to happen at practical temperatures (e.g. mash temperatures).

Here is an eample of an actual enzymatic reaction in the mash. The enzyme is maltase which can split a maltose molecule into two glucose molecules. The reaction consumes one water molecule:

C12H22O11 + H2O -> 2 C6H12O6

With the enzyme maltase the reaction is actually 2 reactions:

C12H22O11 + <Maltase> -> C12H22O11-<Maltase>
C12H22O11-<Maltase> + H2O -> C6H12O6 + <Maltase>

The same is true for other enzymatic reactions in the mash. But for simplicity sake the shorter form of:

substrate1 + substrate2 -> product

Is also used to show the reaction that is happening. The involvement of the enzyme in this reaction is implied


As mentioned earlier. Enzymes are generally very specific in the type of substrate they work on and which reaction they catalyze. A simple model for that behavior is the lock-and-key hypothesis [rsc.org]. In that theory, the enzyme has a shape that fits only a particular substrate. Like the beta amylase which fits only on the non reducing end of a starch chain (Figure 1). If the shape of the enzyme changes significantly due to temperature or pH or inhibitors block the receptor site of the enzyme it cannot react with the substrate and the enzyme becomes inactive.

How temperature effects enzymatic reactions

Figure 2 - The rate of enzymatic reaction increases exponentially as the temperature is increased

The rate of most chemical reactions, including enzymatic reactions, follows the Arrhenius equation [wikipedia.org]:

reaction rate = A * e(-ΔG*/RT)

Where A is the Arrhenius constant, a simple non exponential factor for the reaction rate. ΔG* is the activation energy of the reaction and determines at what temperature the reaction will become "significant". R is the universal gas constant and T is the absolute temperature in Kelvin. To convert a temperature in Celsius into Kelvin 273.15 needs to be added to the Celsius value (I.e. the absolute temperature (0 Kelvin) is -273.15 Celsius). But all that doesn't really matter for understanding this subject. What matters is that the reaction rate of an enzymatic reaction follows an exponential curve (Figure 2). For every 10 C (18F) increase the reaction rate increases 1.2 - 2.5 fold [lsbu.ac.uk].

But if the enzymatic reaction rate follows an exponential curve, why are there different temperature optima for different enzymes?

To answer this question we need to look at another effect that temperature has on enzymes. As mentioned earlier, enzymes are proteins (long chains of amino acids) that are shaped in a particular way which allows them to hold onto their substrate during the reaction. This shape is held in place by weak bonds between different amino acids of the chain. But these bonds are easily broken if the temperature gets too high and the enzyme molecule starts to vibrate too much. This doesn't cause the chain of amino acids to get split, these bonds are much stronger and require much higher temperatures, but the enzyme looses its shape and becomes unable to catalyse the reaction it was made for. It is said to have denatured. Above a critical temperature the rate of denature increases 6 - 36 fold for every temperature increase of 10 C [lsbu.ac.uk]. This is much higher than the increase in the reaction rate and as a result, the productivity of the enzyme will decrease is the temperature is raised past the temperature optimum. Figure 3 shows how the enzyme concentration of a hypothetical enzyme drops for 5 different temperatures.

Figure 3 - The decrease of active enzyme concentration over time for 5 different temperatures for a hypothetical enzyme. The higher the temperature the steeper the decline in the number of enzymes that are able to catalyze reactions
Figure 4 - The increase of the product concentration for 5 different temperatures. The temperature that yields the most product depends on the duration of the reaction. Until t1, the higest temperature actually results in the best enzyme efficiency but then then almost all the enzymes are denatured and the rise of product quickly falls behind the curves for the other temperatures. Up to t2 for example the 60C reaction temperature produced the most product
Figure 5 - The relationship between the reaction temperature and the final product concentration for various reaction times. This graph illustrates how there is no single temperature optimum for a given enzyme. The temperature at which the most product is produced depends on the reaction time. The shorter the reaction time the higher the optimum temperature as short reaction times need sprinters and not marathon runners for to produce the most product

Based one the rate of reaction (Arrhenius equation) and the drop of the active enzyme concentration over time (Figure 3) one can plot the increase of product if unlimited substrate is available. Having unlimited substrate available is not a realistic scenario for mashing but it helps in showing the relationship between the temperature optimum of an enzyme and the reaction time. Figure 4 shows the graphs for the rise in product concentration over time for a hypothetical enzyme at 5 different temperatures. While a high temperature causes a steep initial rise in temperature this high temperature also causes a quick drop in the enzyme concentration and the rise in product concentration quickly levels off and falls behind lower reaction temperatures.

A simple analogy to this behavior is a toy car powered by an electric motor rated for 10V. If the motor is run at 5 volt the car will run very slow but may be able to run for a long time. If run at 10V the car will go faster but only until the motor reached the lifespan it was designed for. Run at 15 V the car will be even faster but the motor is likely to burn out shortly. And if run at 20V the car will get the fastest start of all but won't get far since the motor will burn out quickly. The same happens with the enzymes. At high temperatures they are sprinters and at lower temperatures they are marathon runners.

So far the discussion has only been for virtually unlimited supply of substrate in comparison to the number of enzymes that are available. But this won't be the case in mashing where for example only a limited amount of starch will be available for the amylase enzymes. In this case the temperature optimum changes to a temperature that is good enough to reach full conversion. After that there is no more substrate available and that particular enzymatic reaction will come to a halt. Before that point is reached, the enzymatic reaction will also start to slow down because it becomes harder for the enzymes to find substrate to react with.

The effect of pH

Figure 8 - For each enzyme there is an optimal pH at which it works best. The location and width of that optimum depends on the enzyme. The pH dependent efficiency change is caused by changes of the enzymatic structure and electric charges especially at or around the active sites witch hold on to the substrate during the reaction

The pH of a solution is a logarithmic measure of the freely available H+ ions. The concentration of these ions affects the enzymes in various ways. A change in pH loads to changes in the charges on the enzyme due to the reaction of the H+ ions with the carboxyl or amino functional groups [cuny.edu].

The at high pH (low concentration of H+ in the solution> the carboxyl group disassociates

COOH → COO- + H+

This leaves a negative charge at the site of the carboxyl group and donates a proton H+ to the solution. This reaction is reversed at low pH

At low pH (high concentration of H+ in the solution) the amino functional group binds a proton

NH2 + H+ → NH3+

This results in a positive charge on the site of the amino group. A reaction that is reversed at high pH.

These pH dependent reactions determine the electric charges and as a result the shape of the enzyme and its ability to react with the substrate. As a result a pH exists at which the enzyme will be most efficient performing the reaction it was designed for. On either side of that optimum the effectiveness of the enzyme will decline until it is unable to function anymore.

The change in enzyme activity within 2-3 pH units to either side of the optimum is generally a reversible process [lsbu.ac.uk]. This means that no permanent damage is done to the enzyme. It also means that a suboptimal pH in mashing doesn't necessarily damage the enzymes and that the full enzymatic activity can be restored by adjusting the mash pH into the optimal range, except for the enzymes that have already been denatures. A more severe pH change 3+ units is likely to denature the enzyme due to high stress that the extreme change in the charges place on the structure of the enzyme. This basically makes the enzyme less stable and it denatures at a fairly high rate even below its critical temperature. In some cases strong acidity can also hydrolyze the peptide links (i.e. break the amino acid chain the makes up the enzyme).

When considering pH, it should be noted that the pH of a solution changes with temperature. The rate of change is dependent on the solution itself. For wort and mashes the actual pH is 0.35 units lower at 65 C (150F) than at room temperature 20 C (68 F). At 75 C it is 0.45 units lower [Briggs, 2004].

Inhibitors and cofactors

Some enzymes require the presence of a non protein compound, commonly a metal ion, for the reaction. Without this cofactor the enzyme is not able to catalyze the reaction it was made for. As a result the rate of the enzymatic reaction may also be limited by the concentration and availability of the necessary cofactors. One important cofactor for enzymes needed by the yeast metabolism is for example zink [wikipedia.org]

Inhibitors reduce the reaction rate of the enzymes.




[rsc.org] Chemistry for Biologists - How enzymes work
[lsbu.ac.uk] The effect of temperature on * [lsbu.ac.uk The effect of pH on enzymes, London Southbank University
[wikipedia.org] Arrhenius Equation, Wikipedia.org
[wikipedia.org] Cofactors Wikipedia.org
[cuny.edu] pH and enzymes, City University of New York

Starch

  • where it is found
  • glucose and 1-4/1-6 branches
  • amylose
  • amylopectin
  • starch granule structure

Starch conversion

  • gelatinization
  • active enzymes
  • emzyme temperature and pH optima
  • mash parameters affecting conversion

Proteins

Other enzymes in mashing

Sources