Effect of recovery time on \(\dot{V}{\text{O}}_{2}\)-ON kinetics in humans at the onset of moderate-intensity cycling exercise

Alveolar oxygen uptake (\(\dot{V}{\text{O}}_{{2{\text{A}}}}\)) at the onset of constant-load, moderate-intensity exercise attains the steady-state value (\(\dot{V}{\text{O}}_{{2{\text{ss}}}}\)) following kinetics commonly described as the sum of two mono-exponential responses (Whipp and Ward 1990). The first component (Phase 1, or the cardio-dynamic phase) is related to the rapid increment of pulmonary blood flow (Lador et al. 2006; Loeppke et al. 1981; Yoshida et al. 1993). The second (Phase 2, or primary phase): (i) mirrors the O₂ uptake response of the muscles (\(\dot{V}{\text{O}}_{{2{\text{m}}}}\)) (Grassi et al. 1996, 1998), (ii) appears after a time delay of about 15 s, and (iii) is characterized by a time constant (τ₂) of around 35–45 s in moderately fit healthy subjects (Poole and Jones 2005).

The slowness of \(\dot{V}{\text{O}}_{{2{\text{m}}}}\) kinetics at the onset of exercise implies that the fraction of ATP resynthesized from phosphocreatine (PCr) breakdown before achieving \(\dot{V}{\text{O}}_{{2{\text{ss}}}}\) progressively decreases. The amount of energy derived from the splitting of PCr, the biochemical counterpart of the obligatory O₂ deficit (DefO₂) (Ferretti et al. 2022;  di Prampero 1981; Piiper et al. 1968), fills the gap between the energy requirement of muscle contraction and the energy provided by the aerobic pathway, and is linearly related to \(\dot{V}{\text{O}}_{{2{\text{ss}}}}\). This phenomenon implies that \(\dot{V}{\text{O}}_{{2{\text{m}}}}\) and phosphocreatine concentration ([PCr]) attain the corresponding steady states in a mirror fashion following mono-exponential functions characterized by similar τ (McCreary et al. 1996; Rossiter et al. 1999; Whipp et al. 1999).

The factors regulating the kinetics of \(\dot{V}{\text{O}}_{{2{\text{m}}}}\) and of PCr splitting have been investigated in detail by applying several experimental approaches, and various models of the regulation of the mitochondrial respiration in skeletal muscles have been explained (Meyer 1988; Grassi 2003; Haseler et al. 2004; Kindig et al. 2005). Korzeniewski and Zoladz, for instance, proposed a dynamical model of the respiratory control in muscle fibers based on the quantitative integration of kinetic equations, features of putative enzymes, and biochemical pathways-blocks (Korzeniewski and Zoladz 2001). According to this model, the τ of muscular PCr splitting (τPCr) (and therefore of muscular and alveolar \(\dot{V}{\text{O}}_{2}\) kinetics) is related to the decrease of PCr during the rest-to-work transition (∆PCr) in such a way that τPCr increases linearly as a function of ∆PCr (Korzeniewski and Zoladz 2004). The authors, in agreement with their hypothesis, state that “after the termination of an exercise, if [PCr] did not return to its resting level and a new exercise is started, ∆PCr for this principal exercise will, of course, be smaller than for the previous exercise and therefore t1/2 also will be smaller.” (Fig. 5 and page 708, Korzeniewski and Zoladz 2004). In compliance with the aforementioned theoretical model, experimental data showed a correlation between τPCr at the onset of square-wave exercise and ∆PCr (Greiner et al. 2007). However, more recent findings, based on ³¹P-NMR spectroscopy measures of PCr breakdown at the onset of moderate-intensity, square-wave exercise, did not confirm a direct relationship between ∆PCr and the speed of PCr splitting (Francescato et al. 2008). Instead, these data suggested that [PCr] is the primary controller of oxidative phosphorylation in the skeletal muscle (Walsh et al. 2001) and acts as a sort of energy buffer with a capacitance that is proportional to the PCr content (Meyer 1989). Consequently, τPCr is slower (longer in time), the more prominent the [PCr] prevailing before exercise onset.

At the end of the exercise, the energy requirement and the ATP splitting rate diminish immediately. Nevertheless, \(\dot{V}{\text{O}}_{{2{\text{A}}}}\) gradually decreases following complex kinetics, usually described as the sum of two mono-exponential decays (Cautero et al. 2005). The rapid component of this kinetics mirrors the rate of PCr resynthesis, and the consumed O₂ is utilized to repay the DefO₂ contracted at the onset of the exercise (Piiper and Spiller 1970). The τ of this decay (35–40 s) implies that DefO₂ is completely repaid in about 175–200 s, a time likely sufficient for the full recovery of [PCr]. This recovery time also suggests that if the exercise is resumed before the obligatory DefO₂ has been fully repaid and PCr stores have not been wholly replenished, we start exercising from a lower [PCr]. Suppose the metabolic requirement, i.e., the \(\dot{V}{\text{O}}_{{2{\text{ss}}}}\) elicited by the imposed workload, is unchanged. In that case, we also necessarily imply that the ∆PCr induced by the step transition is lower than that observed when starting from rest. Therefore, the imposition of a square-wave transition at identical workloads, but after different recovery times, might be a simple and effective method to manipulate in a predetermined fashion the pre-transition [PCr] and the ∆PCr of square-wave exercise and to evaluate their effect on the ensuing \(\dot{V}{\text{O}}_{{2{\text{A}}}}\) kinetics.

The possible role of an elevated metabolic rate, dissociated from on \(\dot{V}{\text{O}}_{{2{\text{A}}}}\) kinetics, has been investigated. In one study, for instance, the investigators showed that the dynamic response of \(\dot{V}{\text{O}}_{{2{\text{A}}}}\), and hence of muscular aerobic metabolism, is decelerated when the exercise is resumed starting, during recovery, from a raised metabolic rate (Bowen et al. 2011). This finding was attributed to the recovering muscle's less-favorable energetic status, which directly caused a longer delay of \(\dot{V}{\text{O}}_{{2{\text{A}}}}\) in attaining the steady state.

The present investigation was undertaken to challenge these two opposing hypotheses regarding the behavior of \(\dot{V}{\text{O}}_{{2{\text{A}}}}\) kinetics when the exercise is resumed after different recovery times. The first one predicts that smaller values of starting [PCr] before the onset of the exercise are related to a progressive acceleration of \(\dot{V}{\text{O}}_{{2{\text{A}}}}\) kinetics. The opposite hypothesis states that the raised metabolic rate and the disadvantageous energetic state of the muscle may be associated with a slower \(\dot{V}{\text{O}}_{{2{\text{A}}}}\) kinetics. To this aim, we studied in exercising humans the effects of different recovery times on \(\dot{V}{\text{O}}_{{2{\text{A}}}}\) kinetics during a square-wave cycling exercise transition performed at the same mechanical power. By manipulating the time of recovery, we induced conditions characterized by metabolic rates and [PCr], which are in opposition: for short recovery times, we have high metabolic rates and low [PCr]; the opposite is true for longer times of recovery. In addition, the results may also allow us to evaluate whether the τ₂ of \(\dot{V}{\text{O}}_{{2{\text{A}}}}\) kinetic (from now on, we refer simply to “τ”) is linearly related with the estimated ∆PCr occurring during the transients or not.

The \(\dot{V}{\text{O}}_{2}\) corresponding to GET amounted, on average, to 30.5 ± 10.7 ml kg⁻¹ min⁻¹ and to 47 ± 9.6% of the individual \(\dot{V}{\text{O}}_{{2{\text{peak}}}}\). Mechanical power at GET was 159 ± 41. 4 W. Peak [La]_b after the C square-wave exercise amounted to 2.7 mM ± 0.07 and peak lactate accumulation was 1.7 mM ± 0.07.

In Fig. 2, breath-by-breath \(\dot{V}{\text{O}}_{{2{\text{A}}}}\) values of a typical subject are reported, after superposition, and synchronization, as a function of time from exercise onset during square-wave transitions performed at the same absolute workload but preceded by variable recovery intervals. The control condition C always started from rest, whereas C1 was preceded by 300 s of recovery. The graphs also report the corresponding mono-exponential fitting functions and the estimated τ.

Exercise transitions after the different recovery times started from different metabolic rates. After 30 s of recovery \(\dot{V}{\text{O}}_{{2{\text{A}}}}\) was 1.32 l min⁻¹ ± 0.13; after 60 s, it amounted to 0.89 l min⁻¹ ± 0.13; at 90 s of recovery the subjects resumed exercise when \(\dot{V}{\text{O}}_{{2{\text{A}}}}\) corresponded to 0.66 l min⁻¹ ± 0.12; and after 120 s, \(\dot{V}{\text{O}}_{{2{\text{A}}}}\) was 0.58 l min⁻¹ ± 0.95. In addition, \(\dot{V}{\text{O}}_{{2{\text{A}}}}\) values prevailing before C (0.44 l min⁻¹ ± 0.06) and C1 (0.57 l min⁻¹ ± 0.03) were significantly different (P < 0.01; 95% CI of difference: 0.10–0.17 l min⁻¹).

In Table 1, the average values of the functional gains (G), amplitudes (A), time constants (τ), and time delays (TD) of the \(\dot{V}{\text{O}}_{{2{\text{A}}}}\)-ON kinetics corresponding to the different recovery times are presented together with their standard deviations and the 95% confidence limits of the estimated τ.

Amplitudes of the responses were significantly different in the various conditions. In detail,

Only the amplitudes after 90 s and 120 s of recovery were not significantly different from those assessed after 300 s of recovery (C1).

However, functional gains (grand average 12.1 ml min⁻¹ W⁻¹ ± 0.15), calculated as the ratio between \(\dot{V}{\text{O}}_{{2{\text{A}}}}\) at steady state and workload, and \(\dot{V}{\text{O}}_{{2{\text{ss}}}}\) (grand average: 1.96 l min-1 ± 0.02) were not significantly different for the different times of recovery. Time delays were not affected by the recovery time in any of the cases.

τ of the step transition preceded by the shortest time of recovery (30 s) was significantly larger than the ones of the transitions corresponding to longer recovery times (60 s: P = 0.035, 95% CI of difference: 0.62–14.6 s; 90 s: P = 0.022, 95% CI of difference: 1.67–18.53 s). τ of the transition after the shortest time of recovery (30 s) tended to be larger than the one assessed during exercise performed after 120 s of recovery (P = 0.0905). Likewise, τ assessed after 1 min of recovery tended to be larger than the one estimated during the step transition imposed after 90 s of recovery (P = 0.063). Finally, the τ of the \(\dot{V}{\text{O}}_{{2{\text{A}}}}\)-ON response in C was significantly longer than in C1 (P = 0.044). The decay of τ seemed to decay as a first-order exponential decay of the time of recovery from 30 to 300 s: τ = 109.5 × e^(−t/14.0) + 18.9; r² = 0.32) (Fig. 3).

The results obtained in this investigation showed that the τ of \(\dot{V}{\text{O}}_{{2{\text{A}}}}\)-ON kinetics of a square-wave transition imposed after different recovery times at moderate-intensity exercise decreased with recovery time. Since the amount of PCr resynthesized during recovery is proportional to the volume of O₂ consumed during the rapid phase of the O₂ debt repayment, this would also imply that τ might be affected by the [PCr] existing at the end of recovery or by ∆[PCr] occurring during the subsequent transient. Alternatively, it may be influenced by the raised metabolic rate prevailing before exercise resumption and, hence, on the energetic status of the muscles.

Since τ of \(\dot{V}{\text{O}}_{{2{\text{A}}}}\)-ON kinetics is a close proxy of τPCr, i.e., of the τ of PCr splitting at the onset of exercise, we may speculate that the starting [PCr] and/or ∆[PCr] influence, in the same fashion, also the splitting rate of PCr during the transient.

At variance with other investigations where muscular [PCr] and ∆[PCr] were directly assessed during step exercise transitions (f.i., Francescato et al. 2008), in the present study, muscular [PCr] and ∆[PCr] were not directly measured. Therefore, the paragraphs here below are devoted to discussing the current findings in the light of directly obtained data related to the muscular metabolic condition.