Since Hasselbalch adapted the Henderson equation to the pH notation of Sörenson, we have used the following equation to understand the relationship between respiratory and metabolic acid–base variables:

pH = pK × log [HCO₃ /(0.03 × pCO₂)]   (1)

This is the Henderson–Hasselbalch equation, and it is important to realize what this equation tells us. Anincrease in pCO₂ will result in a decrease in the pH and anincrease in the HCO₃^- concentration. Thus, a patientfound to have a low blood pH, a condition known asacidemia, will either have an increased pCO₂ or a pCO₂that is 'not increased'. In the former circumstance, we classify the disorder as a 'respiratory acidosis'. We use the term 'acidosis' to describe the process resulting in acidemia and 'respiratory' because the apparent cause is an increased pCO₂. This is logical, because carbonic acid results when CO₂ is added to water (or blood), and the resultant decrease in pH is entirely expected. In the latter condition pCO₂ is not increased, and thus there cannot be a respiratory acidosis. We therefore refer to this condition as 'metabolic' because some nonvolatile acid must be the cause of the acidemia. We can reverse the above logic and easily classify simple conditions of alkalemia as either resulting from respiratory or metabolic alkaloses. Thus, equation 1 allows us to classify disorders according to the primary type of acid being increased or decreased. Over time physiology superimposes its effects on simple chemistry and the relationship between pCO₂ and HCO₃^- is altered in order to reduce the alterations in pH. By carefully examining the changes that occur in pCO₂ and HCO₃^- in relationship to each, however, one can discernhighly conserved patterns. In this way rules can be established to allow one to discover mixed disorders and to separate chronic from acute respiratory derangements. For example one such rule is the convenient formula for predicting the expected pCO₂ in the setting of a metabolic acidosis [12]:

pCO₂ = (1.5 × HCO₃^-) + 8 ± 5  (2)

This rule tells us what the pCO₂ should be secondary to the increase in alveolar ventilation that accompanies a metabolic acidosis. If pCO₂ does not change enough or changes too much, we classify the condition as a 'mixed' disorder, with either a respiratory acidosis if the pCO₂ is still too high, or a respiratory alkalosis if the change is too great. This rule, along with others (Table 1) has been recently translated to SBE terminology [7]:

pCO₂ = (40 + SBE) ± 5  (3)

For example, consider the following arterial blood gas sample: pH7.31, pCO₂ 31, HCO₃^- 15, SBE-9.5. Equation 2 tells us that the expected pCO₂ =(1.5×15)+8 ± 5=30.5 ± 5, and in Equation 3 the SBE added to 40 also yields 30.5. The measured pCO₂ of 31 mmHg is consistent with a pure metabolic acidosis (ie no respiratory disorder).

It is also very important to understand what the Henderson-Hasselbach equation does not tell us. First, it does not allow us to discern the severity (quantity) of the metabolic derangement in a manner analogous to the respiratory component. For example, when there is a respiratoryacidosis, the increase in the pCO₂ quantifies the derangement even when there is a mixed disorder. However, the metabolic component can only be approximated by the change in HCO₃^-. Second, Equation 1 does not tell us about any acids other than carbonic acid. The relationship between CO₂ and HCO₃^- provides a useful clinical 'roadmap' to guide the clinician in uncovering the etiology of an acid–base disorder as described above. The total CO₂concentration, and hence the HCO₃^- concentration, is determined by the pCO₂, however, which is in turn determined by the balance between alveolar ventilation and CO₂ production. HCO₃^- cannot be regulated independent of pCO₂. The HCO₃^- concentration in the plasma will always increase as the pCO₂ increases, but this is not an alkalosis. To understand how the pH and HCO₃^- concentration are altered independent of pCO₂, we must look beyond Henderson and Hasselbach.

In order to address the first 'shortcoming' of the Henderson-Hasselbach equation – the inability to quantify the metabolic component – several methods have been devised. In 1948, Singer and Hastings proposed the term 'buffer base' to define the sum of HCO₃^- plus the nonvolatile weak acid buffers (A^-) [13]. A change in buffer base corresponds to a change in the metabolic component. The methods for calculating the change in buffer base were later refined by investigators [14,15] and refined further by others [16,17,18] to yield the base excess methodology. Base excess is the quantity of metabolic acidosis or alkalosis, defined as the amount of acid or base that must be added to a sample of whole blood in vitro in order to restore the pH of the sample to 7.40 while the pCO₂ is held at 40 mmHg [15]. Although this calculation is quite accurate in vitro, inaccuracy exists when applied in vivo in that base excess changes with changes in pCO₂ [19,20]. This effect is understood to be due to equilibration across the entire extracellular fluid space (whole blood + interstitial fluid). When the base excess equation is modified to account for an 'average' content of hemoglobin across this entire space, a value of 5 g/dl is used instead, and this defines the SBE. It should be pointed out that this value does not represent the true content of hemoglobin suspended in the volume of whole blood together with interstitial fluid, but rather is an empiric estimate that improves the accuracy of the base excess. It can be argued that the entire extracellular fluid space is involved in acid–base balance, because this fluid flows through blood vessles and lymphatics, mixing constantly [21]. Thus, the value of SBE is that it quantifies the change in metabolic acid–base status in vivo. It is of interest that base excess is only accurate in vivo when it assumes a constant hemoglobin concentration.

However, the base excess approach does not address the second problem associated with using the Henderson-Hasselbach equation alone (ie it still does not tell us about the mechanisms of metabolic acid–base balance). For example the body does not 'regulate' the SBE. It is not a substance that can be excreted in the feces or reabsorbed from the proximal tubule. Similarly, HCO₃ ^- is not a strong acid or base and its addition to or removal from the plasma cannot be translated into changes in SBE. This not to say that changes in SBE and HCO₃^- do not correlate closely, because they do. However, correlation and causation are not the same thing. The difference has traditionally been ascribed to the effects of 'buffering', the argument being that stong acid (or base), quantified by SBE, is 'buffered' by plasma proteins, hemoglobin, and finally by HCO₃^-. The resulting changes in HCO₃^-and pH are then a result of this buffering process. These buffers are actually weak acids, however, and their addition to plamsa both decreases the pH and increases the responsiveness to pCO₂ (Fig. 1). Furthermore, as explained by Stewart [6,9], the fundamental physical-chemical properties of biologic solutions dictate much of this so-called 'buffering'.

CO₂ is an independent determinant of pH and is produced by cellular metabolism or by the titration of HCO₃ - by metabolic acids. Normally, alveolar ventilation is adjusted to maintain the arterial pCO₂ between 35 and 45 mmHg. When alveolar ventilation is increased or decreased out of proportion to pCO₂ production, a respiratory acid–base disorder exists. CO₂ production by the body (at 220 ml/min) is equal to 15000 mmol/day of carbonic acid [23]. This compares with less than 500 mmol/day for all nonrespiratory acids. The respiratory center, in response to signals from pCO₂, pH, and partial oxygen tension, as well as some from exercise, anxiety, wakefulness, and others, controls alveolar ventilation. A precise match of alveolar ventilation to metabolic CO₂ production attains the normal arterial pCO₂ of 40 mmHg. Arterial pCO₂ is adjusted by the respiratory center in response to altered arterial pH produced by metabolic acidosis or alkalosis in predictable ways.

When CO₂ elimination is inadequate relative to the rate of tissue production, pCO₂ will increase to a new steadystate that is determined by the new relationship between alveolar ventilation and CO₂ production. Acutely, this increase in pCO₂will increase both the H⁺ and the HCO₃^- concentrations according to the Henderson-Hasselbach equation (Equation 1). Thus, this change in HCO₃^- concentration is mediated by chemical equilibrium, and not by any systemic adaptation. Similarly, this increased HCO₃^- concentration does not 'buffer' H⁺ concentration. There is no change in the SBE. Tissue acidosis always occurs in respiratory acidosis, because CO₂ diffuses into the tissues. If the pCO₂ remains increased the body will attempt to compensate by altering another independent determinant of pH, namely the SID.

Blood plasma contains numerous ions. These ions can be classified both by charge, positive 'cations' and negative 'anions', as well as by their tendency to dissociate in aqueous solutions. Some ions are completely dissociated in water, for example, Na⁺, K⁺, Ca²⁺, Mg²⁺, and Cl^-. These ions are called 'strong ions' to distinguish them from 'weak ions' (eg albumin, phosphate and HCO₃^-), which can exist both as charged (dissociated) and uncharged forms. Certain ions such as lactate are so nearly completely dissociated that they may be considered strong ions under physiologic conditions. In a neutral salt solution containing only water and NaCl, the sum of strong cations (Na⁺) minus the sum of strong anions (Cl^-) is zero (ie Na⁺ = Cl^-). In blood plasma, however, strong cations (mainly Na⁺) outnumber strong anions (mainly Cl^-). The difference between the sum of all strong cations and all strong anions is known as the SID. SID has a powerful electrochemical effect on water dissociation, and hence on H⁺ concentration. As SID becomes more positive, H⁺, a 'weak' cation, decreases (and pH increases) in order to maintain electrical neutrality (Fig. 2).

In healthy humans, the plasma SID is between 40 and 42 mmol/l, although it is often quite different in critically ill patients. According to the principle of electrical neutrality, blood plasma cannot be charged, so the remaining negative charges balancing the SID come from CO₂ and theweak acids (A^-) and, to very small extent, from OH^-. At physiologic pH, the contribution of OH^- is so small (nmol range) that it can be ignored. The total weak acid concentration (mainly albumin and phosphate) can be considered together and for convenience is abbreviated A_TOT, where AH + A^- = A_TOT. The SID of a blood sample can be estimated from the value of the remaining negative charge, because SID-(CO₂ +A ^-)=0. This estimate of SID has been termed the 'effective' SID [24], but it is really no different from buffer base described over half a century ago [13]. Thus SID and buffer base are mirror images of each other. Recall that SBE is essentially the change in buffer base in vivo, and hence SBE defines the change in SID from the equilibrium point where pH=7.4 and pCO₂ = 40 mmHg [8].

An alternative estimate of SID is as follows: (Na⁺ + K⁺ + Ca²⁺+ Mg²⁺) – (Cl^- + lactate^-). This is often referred to as the 'apparent' SID with the understanding that some 'unmeasured' ions might also be present [24]. Neither effective SID nor the apparent SID are perfect estimates of the true SID. Blood samples from patients may contain unmeasured strong ions (eg sulfate, ketones) making the apparent SID an inaccurate estimate of SID. Similarly, these patients may have abnormal weak ions (eg proteins) that will make the effective SID inaccurate. In healthly humans, however, the apparent SID and the effective SID are nearly identical, and are thus valid estimates of SID [24]. Furthermore, when the apparent SID and the effective SID are not equal, a condition we have referred to as the strong ion gap (SIG), where apparent SID – effective SID = SIG, abnormal strong and/or weak ions must be present [25]. The SIG is positive when unmeasured anions exceed unmeasured cations, and negative when unmeasured cations exceed unmeasured anions. Unexplained anions, and in some cases cations, have been found in the circulation of patients with a variety of diseases [25,26,27,28] and in animals under experimental conditions [29].

The SIG is not the same as the anion gap (AG). Normally, the SIG is zero, whereas the AG is 8–12mmol/l. The AG is an estimate of the sum of SIG + A^-. Thus, subtracting A^- from the AG approximates the SIG. A convenient and reasonably accurate way to estimate A^- is to use the following formula [30]:

2 (albumin g/dl) + 0.5 (phosphate mg/dl)  (4)

or for international units:

0.2 (albumin g/l) + 1.5 (phosphate mmol/l)  (5)

Note that the 'normal' AG for a person with no unmeasured anions or cations in their plasma is equal to A^-, such that AG - A^- = SIG = 0. This technique allows one to 'calibrate' the AG for patients with abnormal albumin and/or phosphate concentrations.

In order to alter the SID, the body must affect a change in the relative concentrations of strong cations and strong anions. The kidney is the primary organ that affects this change. However, the kidney can only excrete a very small amount of strong ion into the urine each minute, and several minutes to hours are therefore required to impact significantly on the SID. The handling of strong ions by the kidney is extremely important because every Cl^- ion filtered but not reabsorbed increases the SID. Because most of the human diet contains similar ratios of strong cations to strong anions, there is usually sufficient Cl^-available for this to be the primary regulating mechanism. This is particularly apparent when we consider that renal Na⁺ and K⁺ handling are influenced by other priorities (eg intravascular volume and plasma K⁺ homeostasis). Accordingly, 'acid handling' by the kidney is generally mediated through Cl^- balance. How the kidney handles Cl^- is obviously very important. Traditional approaches to this problem have focused on H⁺ excretion and have emphasized the importance of NH₃ and its add-on cation NH₄⁺. H⁺ excretion per se is irrelevant, however, because water provides an essentially infinite source of free H⁺. Indeed the kidney does not excrete H⁺ any more as NH₄+ than it does as H₂O. The purpose of renal ammoniagenesis is to allow the excretion of Cl^- without excreting Na⁺ or K⁺. This is achieved by supplying a weak cation (NH₄⁺) to excrete with Cl^-.

Thus, NH₄⁺ is important to systemic acid–base balance,not because of its carriage of H⁺ or because of its direct action in the plasma (normal plasma NH₄⁺ concentration is <0.01mmol/l), but because of its 'coexcretion' with Cl^-. Of course, NH₄⁺ is not only produced in the kidney. Hepatic ammoniagenesis (and also glutaminogenesis) is important for systemic acid–base balance and, as expected, it is tightly controlled by mechanisms that are sensitive to plasma pH [31]. Indeed this reinterpretation of the role of NH₄⁺ in acid–base balance is supported by the evidence that hepatic glutaminogenesis is stimulated by acidosis [32]. Nitrogen metabolism by the liver can result in either urea, glutamine or NH₄⁺. Normally, the liver does not release more than a very small amount NH₄⁺, but rather incorporates this nitrogen into either urea or glutamine. Hepatocytes have enzymes to enable them to produce either of these end products, and both allow for the regulation for plasma NH₄⁺ at suitably low levels. The production of urea or glutamine has significantly different effects at the level of the kidney. This is because glutamine is used by the kidney to generate NH₄⁺ and facilitatethe excretion of Cl^-. Thus, the production of glutamine can be seen as having an alkalinizing effect on plasma pH because of the way in which the kidney utilizes it.

Further support for this scenario comes from the recent discovery of an anatomic organization of hepatocytes according to their enzymatic content [33]. Hepatocytes with a propensity to produce urea are positioned closer to the portal venule, and thus have the first chance at the NH4⁺delivered. Acidosis inhibits ureagenesis, however, and under these conditions more NH₄⁺ is available for the downstream hepatocytes that are predisposed to produce glutamine. Thus, the leftover NH₄⁺ is 'packaged' as glutamine for export to the kidney, where it is used to facilitate Cl^- excretion and hence increases the SID.

The gastrointestinal tract also has important effects on the SID. Along its length, the gastrointestinal tract handles strong ions quite differently. In the stomach, Cl^- is pumped out of the plasma and into the lumen, reducing the SID of the gastric juice and thus reducing the pH. On the plasma side, SID is increased by the loss of Cl^- and the pH is increased, producing the so-called 'alkaline tide' that occurs at the beginning of a meal when gastric acid secretion is maximal [34]. In the duodenum Cl^- is reabsorbed and the plasma pH is restored. Normally, only slight changes in plasma pH are evident because Cl^- is returned to the circulation almost as soon as it is being removed. If gastric secretions are removed from the patient, however, either by suction catheter or vomiting, Cl^- will be progressively lost and the SID will steadily increase. It is important to realize that it is the Cl^- loss, and not the H⁺ that is the determinant of plasma pH. Although H⁺ is 'lost' as HCl, it is also lost with every molecule of water removed from the body. When Cl^- (a strong anion) is lost without loss of a strong cation, the SID is increased and therefore the plasma H⁺ concentration is decreased. When H⁺ is 'lost' as water (HOH) rather than HCl, there is no change in the SID and hence no change in the plasma H⁺ concentration.

In contrast to the stomach, the pancreas secretes fluid into the small intestine that has a SID much higher than that of plasma and is very low in Cl^-. Thus, the plasma perfusing the pancreas has its SID decreased, a phenomenon that peaks about 1 h after a meal and helps counteract the alkaline tide. If large amounts of pancreatic fluid are lost, for example from surgical drainage, an acidosis will result as a consequence of the decreased plasma SID. In the large intestine, fluid also has a high SID because most of the Cl^- has been removed in the small intestine and the remaining electrolytes are mostly Na⁺ and K⁺. The body normally reabsorbs much of the water and electrolytes from this fluid, but when severe diarrhea exists large amounts of cations can be lost. If this loss is persistent, the plasma SID will decrease and acidosis will result. Finally, whether the gastrointestinal tract is capable of regulating strong ion uptake in a compensatory manner has not been well studied. There is some evidence that the gut may modulate systemic acidosis in experimental endotoxemia by removing anions from the plasma [35]. The full capacity of this organ to affect acid–base balance is unknown, however.