Abstract
In rod photoreceptors, deactivation of the light-activated G-protein-coupled receptor rhodopsin (R*) is initiated by phosphorylation and completed through subsequent binding of visual arrestin (Arr1). The in vivo kinetics of these individual interactions have proven difficult to determine with precision since R* lifetime is much shorter than the lifetimes of downstream G-protein and effector molecules. Here, we have used a transgenic mouse line with accelerated downstream deactivation kinetics to reveal the contribution of Arr1 binding to the overall time course of rhodopsin deactivation. Photoresponses revealed that the lifetime of R* is significantly increased in rods that express half of the normal amount of Arr1, in a manner consistent with a twofold decrease in the rate of Arr1 binding across a wide range of flash strengths. A basic model of photoresponse deactivation consistent with established photoreceptor biochemistry shows that R* phosphorylation and Arr1 binding occur with a time constant of ∼40 ms in wild-type mouse rods, much faster than previous estimates.
Introduction
In nearly all eukaryotic cells, deactivation of G-protein-coupled receptors determines the balance between signal amplification and timely response recovery. In the G-protein cascade of retinal rods, photoexcited rhodopsin (R*) activates the G-protein transducin (Gtα) at a rate of several hundred per second (Heck and Hofmann, 2001; Arshavsky et al., 2002) throughout its active lifetime, providing the amplification needed for single-photon detection. Prolonging R* lifetime by interfering with deactivation mechanisms, which include phosphorylation by GRK1 and final quench by the binding of visual arrestin (Arr1), slows recovery of the outer segment light response (Xu et al., 1997; Chen et al., 1999; Mendez et al., 2000; Doan et al., 2006; Chan et al., 2007). However, the normal active lifetime of R* as determined by these deactivation mechanisms remains one of the fundamental unsolved puzzles in phototransduction.
Defining the individual contributions of phosphorylation and Arr1 binding to R* deactivation in normal rods has been challenging because phosphorylation both reduces R* activity and increases the affinity for Arr1 binding (Palczewski et al., 1992; Krupnick et al., 1997; Xu et al., 1997; Gurevich, 1998; Gibson et al., 2000; Vishnivetskiy et al., 2007). Overexpression of GRK1 has no effect on the amplitude or time course of the light response (Krispel et al., 2006; Whitcomb et al., 2009), indicating that GRK1 expression does not rate-limit R* deactivation. Underexpression of Arr1 similarly has no consequences for the duration of the single-photon response (Xu et al., 1997), suggesting that Arr1 binding also does not rate-limit R* deactivation. The apparent lack of effect of both GRK1 and Arr1 expression on the time course of the dim flash response might arise because R* deactivation is much faster than the deactivation of downstream G-protein/effector molecules (Gtα/PDE) (Krispel et al., 2006; Burns and Pugh, 2009; Chen et al., 2010). Thus, we reasoned that the kinetics of the dim flash response would be more sensitive to small changes in R* lifetime in rods with accelerated Gtα GTPase activity, such as those that overexpress the RGS9 complex (Krispel et al., 2006).
To test this idea, we have recorded from rods with normal and reduced Arr1 expression in the RGS9-overexpression (RGS9-ox) background. Our results in both wild-type and RGS9-ox backgrounds support the conclusion that decreased Arr1 expression indeed leads to a slowing of R* deactivation and provide new estimates of the rate of phosphorylation and Arr1 binding in intact mouse rods.
Materials and Methods
Use of experimental animals.
Mice were cared for and handled following an approved protocol from the Institutional Animal Care and Use Committee of the University of California, Davis, and in compliance with National Institutes of Health guidelines for the care and use of experimental animals. Control mice in this study consisted of adult wild-type C57B/6 mice (Charles River) and R9AP138 transgenic mice (fourfold overexpressors; Krispel et al., 2006). Mice hemizygous for Arr1 were obtained by breeding each of these control strains with Arr1−/− mice (Xu et al., 1997). Genotypes were determined by PCR analysis as previously described (Xu et al., 1997; Krispel et al., 2006).
Isolation of rod outer segments.
Approximately 12 retinas were harvested in darkness from dark-adapted mice of each genotype (WT or Arr1+/−) and vortexed in 2% OptiPrep (Sigma). This preparation was centrifuged through a gradient of 8%, 12%, 16%, and 20% OptiPrep for 20 min, which resulted in three visibly distinct bands of tissue in the gradient. The bottom two bands were collected, filtered, pelleted, and washed in Ringer's solution (130 mm NaCl, 3.6 mm KCl, 2.4 mm MgCl2, 1.2 mm CaCl2, 10 mm HEPES, and 0.2 mm EDTA). The final product was stored in the dark at −80°C.
Quantitative Western blotting.
A freshly isolated, dark-adapted mouse retina or a frozen pellet of isolated mouse ROS was homogenized in Ringer's solution and maintained at 4°C in the dark. An aliquot of the homogenate was then added to a solution containing 70 mm n-octylglucoside and 50 mm hydroxylamine, pH 7.4. The rhodopsin content of the solution was determined by measuring the absorptivity at 500 nm before and after a full bleach assuming the extinction coefficient ε = 40,500. The remaining homogenate was then diluted in sample buffer so that the final concentration of rhodopsin was 1.0 μm. To facilitate comparisons, tissue samples from WT and transgenic retinas were processed together for Western blots: samples were subjected to twofold serial dilutions, separated by SDS-PAGE, and transferred to PVDF membrane (Bio-Rad). Blots were incubated with either rabbit anti-Arr1 (178605, Calbiochem), mouse anti-RK (MA1-720, Affinity Bioreagents), or rabbit anti-Gtα (sc-389, Santa Cruz Biotechnology) and the appropriate secondary antibodies conjugated to IR dyes (Invitrogen). Signals were detected and quantified with a Li-Cor Odyssey system.
Electrophysiology.
All mice were reared in 12 h cyclic light. On the day of an experiment, an adult mouse that had been dark adapted overnight was killed with CO2 and decapitated under infrared light. One retina was dissected and processed for Western blotting, and the other retina was stored in Leibovitz's medium (L-15; Invitrogen) on ice for suction electrode recordings in bicarbonate-buffered Locke's solution at 36 ± 1°C as previously described (Keresztes et al., 2004). Because a recent report promoted the idea that R* lifetime is longer than Gtα/PDE in rod responses recorded in Ames' medium at 30°C, some experiments were executed with the precise storage and recording conditions described by the protocol in the Materials and Methods of that report (Doan et al., 2009). The results of these experiments are reported in the supplemental material (available at www.jneurosci.org).
The average number of photoisomerizations per flash (n) was calculated with variance-to-mean analysis from an ensemble of at least 25 responses to dim flashes, which by definition had amplitudes that were <20% of the maximal response amplitude (Rieke and Baylor, 1998). The average single-photon response was determined by dividing the average dim flash response by n.
We empirically calculated the effective collecting area for each rod by dividing n by the flash strength [in photons per square micrometer (Baylor et al., 1979)]. The average effective collecting area of wild-type rods (0.34 ± 0.03 μm2, n = 18) was slightly larger (p < 0.03) than those of Arr1+/− (0.24 ± 0.03 μm2, n = 18), RGS9-ox (0.22 ± 0.02 μm2, n = 16), and Arr1+/−RGS9-ox rods (0.24 ± 0.03 μm2, n = 33). For each rod, the effective collecting area was multiplied by a known flash strength to calculate the number of R*/flash for Figure 4.
Calculation of single-photon response time-dependent variance.
To identify individual single-photon responses (SPRs), the average dim flash response was converted to a template (Baylor et al., 1979) by normalizing the peak amplitude to 1.0 and truncating the response after the first 250 ms following the flash. Each individual dim flash response was assigned a scaling factor determined by the value of the cross-correlation of the response with the template at the time point of the flash. A histogram was constructed from these scaling factors, yielding a Poisson distribution, and SPRs were differentiated from failures and multiple photoisomerizations by the local minima on either side of the first peak not centered at zero (Rieke and Baylor, 1998). The response average and time-dependent variance were calculated for the isolated SPRs of each rod. Four Arr1+/− and four wild-type rods were selected so that the subpopulation mean SPRs had similar peak amplitudes. The average time-dependent variances for these subpopulations are shown in Figure 2C.
Determination of time required for dominance: defining “sufficiently late times” for measuring deactivation kinetics.
The recovery of the rod OS photoresponse in dim and saturating flash regimes follows the decline of Gtα/PDE, which was first approximated as the convolution of two exponentials: Here, τR and τE are time constants for the decay of R* and Gtα/PDE, while νRE is the rate constant for Gtα/PDE activation by R* (Pugh and Lamb, 1993). Under this framework, E*(t) approximates a single-exponential decay function with a time constant τD = τE at sufficiently late times (Nikonov et al., 1998). We developed a mathematical method to define “sufficiently late times” given values of τR, τE, and a term for the experimental uncertainty (Eq. 4; supplemental material, available at www.jneurosci.org). Once dominance is established, Equation 1 reduces to the following: The vertical shift in saturation times (Δt) resulting from an increase in τR associated with underexpression of Arr1+/− (Fig. 4) can be used to calculate the time constant for the decay of R* in Arr1+/− rods by setting E*(t;τRwt) = E*(t + Δt;τR+/−): The small difference between τRwt and τR+/− permitted by Equation 3 partially motivated our adoption of the two-time constant model for R* deactivation (Eq. 5).
Results
Arr1 concentration is reduced in Arr1+/− rod outer segments
Previous quantifications of Arr1 content in Arr1+/− retinas have resulted in values varying from 33% to 47% of that found in WT retinas (Xu et al., 1997; Hanson et al., 2007a; Doan et al., 2009), and immunohistochemical quantification of Arr1 compartmentalization suggested that a similar proportion of the overall Arr1 content is localized to the OS in rods with normal and reduced Arr1 expression (Hanson et al., 2007a). To understand the effects of reduced Arr1 expression on rod flash responses, it was first necessary to quantify the levels of Arr1 protein in the dark-adapted OS of the Arr1+/− mice in our colony. Thus, we performed quantitative Western blots on both whole retinal homogenates and purified rod outer segments (ROS) from dark-adapted Arr1+/− mice. We found that Arr1 expression in retinas of Arr1+/− mice was half that of WT retinas (ratio to WT expression = 0.51 ± 0.01 for Arr1+/−; n = 4) (Fig. 1A,D). A similar test performed on purified ROS from Arr1+/− mice demonstrated that a reduction in overall Arr1 expression results in a reduction in OS Arr1 content of similar scale (supplemental Fig. S1, available at www.jneurosci.org as supplemental material), although this purification method is unlikely to provide a precise quantification of Arr1 since it is vulnerable to inner segment contamination and therefore less reliable than previous results (Hanson et al., 2007a). We conclude that the amount of Arr1 in the OS is a fixed percentage of the cell's total Arr1 protein, and thus there does not seem to be a mechanism to maintain a fixed ratio of Arr1:rhodopsin in dark-adapted OS.
To test whether changes in the expression of GRK1 and Gtα might compensate for the reduction of Arr1 in Arr1+/− rods, we performed quantitative Western blots of wild-type and Arr1+/− retinas, but found no significant differences (data not shown), consistent with previous reports (Doan et al., 2009). Furthermore, Arr1 levels in RGS9-overexpressing rods were normal (ratio to WT expression = 1.10 ± 0.05; p = 0.25 compared to WT; n = 5) (Fig. 1B,D), and Arr1 was similarly reduced in Arr1+/−RGS9-ox retinas as in Arr1+/− retinas (ratio to WT expression = 0.56 ± 0.05; n = 5; p = 0.37 compared to Arr1+/−) (Fig. 1C,D). The results of these Western blot experiments led us to conclude that the effects of Arr1 underexpression could be best addressed by returning to electrophysiology, first to develop a more complete characterization of the responses of Arr1+/− rods, and then to test whether the normally slower Gtα/PDE deactivation masks the consequences of a reduced rate of Arr1-R* binding in rods with reduced Arr1 expression.
Reduced Arr1 expression slows rhodopsin deactivation
Consistent with earlier reports under similar conditions (Xu et al., 1997), individual flash families from WT and Arr1+/− rods were qualitatively similar (Fig. 2A). To more directly compare the response time courses, we calculated the average SPRs with variance-to-mean analysis from a large number (n > 25) of dim flash responses. An overlay of the population mean SPRs of WT and Arr1+/− rods revealed them to be nearly identical (Fig. 2B). Accordingly, the kinetic parameters of the dim flash response (time to peak, integration time, and time constant of recovery), which do not rely on variance-to-mean analysis, were all approximately the same for these rods (Table 1) (p > 0.3 for all metrics). Furthermore, the time-dependent variability of isolated SPRs in WT and Arr1+/− rods was similar in waveform, suggesting that SPR reproducibility is unaffected by underexpression of Arr1 (Fig. 2C). Thus, our more detailed characterization of Arr1+/− dim flash responses failed to reveal any effects of reduced Arr1 expression.
To test the idea that slowed Arr1 binding in Arr1+/− rods is obscured by still slower Gtα/PDE deactivation, we recorded from Arr1-deficient rods that expressed the RGS9 complex at fourfold higher levels than normal (RGS9-ox; Krispel et al., 2006). In general, Arr1+/−RGS9-ox responses were larger and longer lasting than those of RGS9-ox rods, as revealed by representative flash families in Figure 3A. The population average SPR of Arr1+/−RGS9-ox rods continued to rise after the RGS9-ox SPR reached a peak (Table 1) (p < 0.03) (Fig. 3B,C). The rising phases of the average SPRs, which indicate the gain of the phototransduction cascade, followed a similar initial trajectory, as determined by the overlapping error bars (SEM) in Figure 3C and by measurement of the rate of change of the light-activated PDE activity (Pugh and Lamb, 1993). The longer time to peak therefore resulted in a larger SPR amplitude in the Arr1-underexpressing rods (Table 1) (p < 0.001) (Fig. 3B). Because the dark currents in these rods were indistinguishable (p = 0.4) (Table 1), an increased SPR amplitude suggests that a reduction of OS Arr1 content does lead to a reduced rate of Arr1-R* binding, and a longer average lifetime of R*.
Further evidence for a longer R* lifetime in Arr1-deficient rods is provided by analysis of the recovery of RGS9-ox and Arr1+/−RGS9-ox dim flash responses. The final falling phase of the average dim flash response can be fit with a single-exponential function whose time constant τrec has a value of ∼230 ms in WT and Arr1+/− rods (Table 1). This 230 ms value reflects the time constant for Gtα/PDE deactivation and is reduced to 76 ms in rods that fourfold overexpress RGS9 (Krispel et al., 2006). Accelerated responses in RGS9-ox rods should reflect the time course of R* catalytic activity more closely than those of WT rods, and one would therefore expect that a sufficiently prolonged R* lifetime in the RGS9- ox background would increase τrec. Indeed, Arr1+/−RGS9-ox responses recovered more slowly than RGS9-ox responses, with an average τrec of 109 ms (Fig. 3B, Table 1) (p < 0.003). Thus, we conclude that the reduced Arr1 levels in Arr1+/−RGS9-ox rods causes slowed rhodopsin deactivation.
The extent to which rhodopsin deactivation is slowed when Arr1 is underexpressed can be constrained by measurements of the dominant time constant of recovery for saturating flashes. This time constant, τD, is given by the slope of the linear relationship between the time that bright flash responses remain in saturation (Tsat; >90% current suppression) and the natural logarithm of the number of photoisomerizations produced by the flashes (Pepperberg et al., 1992). In a previous study, we found that τD, like τrec, undergoes a shift from ∼200 ms to ∼80 ms in RGS9-ox rods (Krispel et al., 2006). In the present study, we found that τD is not larger for Arr1+/−RGS9-ox responses than for RGS9-ox responses (Fig. 4A, Table 1). Therefore, recovery of both Arr1+/−RGS9-ox and RGS9-ox saturating responses is dominated by the same ∼80 ms time constant.
It is important to point out that we used no particular criteria for including or excluding cells in our analyses of either τD or τrec; nevertheless, it was not always possible to obtain sufficient numbers of flash responses to determine both of these metrics in all cells. For the specific set of rods in which τrec and τD were both determined, the average values of τrec were 66 ± 6 ms (n = 23) and 102 ± 7 ms (n = 19) for RGS9-ox and Arr1+/−RGS9-ox rods, respectively (p < 0.001), and the average values of τD were 74 ± 3 ms and 79 ± 6 ms (p = 0.4). Why is there an increase in dim flash τrec for Arr1+/−RGS9-ox rods and yet no corresponding increase in τD, when there is normally excellent correspondence between these two metrics (Chen et al., 2000), even when Gtα/PDE deactivation has been dramatically speeded (Krispel et al., 2006; Chen et al., 2010; our results, Table 1)? The difference between τrec and τD in Arr1+/−RGS9-ox rods can be explained by careful examination of the time intervals over which the two metrics are determined. Because both R* and Gtα/PDE deactivation proceed simultaneously, one must wait until “sufficiently long times” for the slower of these two steps to dominate response recovery, with the time required for dominance determined by the rates of R* and Gtα/PDE deactivation (Nikonov et al., 1998). Our measurements of τrec begin as early as 180 ms after the flash in Arr1+/−RGS9-ox rods, while measurements of τD typically span the interval of 250–400 ms after the flash. While this latter time interval clearly fits the description of “sufficiently late times” because of the linearity of the semilog Tsat relation (Fig. 4A), this criterion may not be met for the measurement of τrec when R* lifetime has been lengthened.
To investigate this idea further, we approximated the time course of the light-driven PDE activity [E*(t)] underlying the photoresponses as the convolution of two exponential decay functions describing R* and Gtα/PDE decay (τR and τE, respectively) and developed a mathematical relationship that defines the time tc at which dominance of the slower time constant is established (see Materials and Methods). A numerical value for tc can be fully determined by choosing values of τR, τE, and an error term (α = 0.1) reflecting the fractional uncertainty in our measurements of τD: Letting τD = τE = 80 ms for rods that overexpress RGS9, a value of τR = 30 ms yields tc = 83 ms when Equation 4 is solved numerically for tc. However, when the time constant for R* decay is doubled (τR = 60 ms) to reflect a 50% decrease in Arr1 expression, Equation 4 yields tc = 271 ms. This indicates that one would have to wait 271 ms after the flash in order for the final recovery phase of the photoresponse (τrec) to reflect τE in the Arr1+/−RGS9-ox rods; by this time, the response has already recovered. In other words, τrec only reflects the slower of τR and τE if the two time constants are sufficiently different from each other. Importantly, when R* deactivation is normal (τR = 30 ms), tc is sufficiently short (83 ms) so that τrec does match τD, as observed in RGS9-ox rods. Thus, the dissimilarity of τrec and τD in Arr1+/−RGS9-ox rods (p < 0.01) further supports the conclusion that R* deactivation is slowed in rods that underexpress Arr1, and that this prolonged R* lifetime is still shorter than the 80 ms lifetime of Gtα/PDE.
Although the slopes (τD) of the Tsat relations were the same, the absolute times that responses remained in saturation were consistently longer in Arr1+/−RGS9-ox than in RGS9-ox rods, resulting in an ∼40 ms vertical offset of the Tsat values (Fig. 4A). Remarkably, examination of the Tsat relations of Arr1+/− and wild-type responses (Fig. 4A, bottom) showed the same ∼40 ms vertical offset (Fig. 4B). This offset could not be explained by subtle differences in the rods' collecting areas or flash sensitivities, which were directly measured in each cell (see Materials and Methods). The fact that Arr1 underexpression resulted in the same 40 ms offset in both WT and RGS9-overexpressing backgrounds suggests that the reduced Arr1 expression slowed rhodopsin deactivation to the same extent in the two genetic backgrounds.
Deduction of the rates of phosphorylation and Arr1 binding for rhodopsin deactivation
While τD is a convenient measure of the slowest, “dominant” time constant, the absolute time that a bright flash response remains in saturation can provide information about R* decay (i.e., the “nondominant time constant”) (Nikonov et al., 2000). All other parameters being equal, the increase in saturation times that we observed in Arr1-underexpressing rods limits the magnitude of the increase in the lifetime of R*. For the two-time constant model discussed above (Eq. 3 in Materials and Methods), the 40 ms change in the absolute time in saturation is consistent with only a small increase in R* lifetime (8–17% increase in R* lifetime from a WT value between 80 and 20 ms). However, since R* deactivation is a multistep process in which Arr1 binding occurs only after phosphorylation has partially reduced R* activity (Gurevich, 1998; Gibson et al., 2000; Vishnivetskiy et al., 2007), such a simple first-order scheme that is entirely dependent on Arr1 binding seems inappropriate. Instead, we adopted a double-exponential scheme for R* deactivation, with the two components representing the time courses of phosphorylation and Arr1 binding, and assumed that underexpression of Arr1 would affect only Arr1 binding.
Thus, the centerpiece of our revised model is a Gtα/PDE pulse [E*(t)] defined by three time constants corresponding to the time courses of R* phosphorylation (τk), R* quench by Arr1 (τa), and Gtα/PDE deactivation (τE): The star (*) in Equation 5 indicates a convolution operation. Because τE is experimentally determined as the dominant time constant of recovery, the only free parameters in this equation are τk and τa. The amplitude ratio of the contributing terms (Aa/Ak) is determined by the values of the time constants τk and τa and the observed 40 ms increase in saturation times (Fig. 4; see Materials and Methods). The rate constant for the activation of Gtα/PDE by R*, νRE, affects the amplitude of E*(t) but has no consequence for our results relating to the time course of recovery. The values of τk and τa were each allowed to vary between 0 and 80 ms, and for each pair, a numerical score was calculated based upon the similarity of the final falling phases of the modeled E*(t) pulses and the observed τrec data (Fig. 5A) over the same time window. Our Arr1+/− data provided strong constraints for this model, with best-fitting values τk = 36 ms and τa+/− = 67 ms (for details on fitting process, see supplemental material, available at www.jneurosci.org). Thus, when Arr1 levels are one-half of normal, the time constant for R* phosphorylation is 36 ms, and that of Arr1 binding is 67 ms. If Arr1 binding becomes approximately twofold faster when Arr1 expression is doubled to the WT level, then the representation of R* decay in our model reduces to a single-exponential function with τawt = τk = 36 ms for responses of rods with normal Arr1 expression. Indeed, this parameterization produced E*(t) time courses that were statistically equivalent to the experimental measurements of τD and τrec from WT and RGS9-ox rods (Fig. 5). To further test whether the double-exponential scheme for R* deactivation was sufficient to explain the experimental observations, the fitting procedure was performed a second time as described above, except that the assumption τawt = τk was replaced with the assumption τa+/− = 2τawt, so that the free parameters for this fitting procedure were τk and τawt. Importantly, the best-fit values determined with this alternate assumption were extremely close to the values reported for the first fitting procedure (τk = 36 ms, τa+/− = 2τawt = 68 ms). The score for the pair of best-fit values was slightly worse than that produced by the parameter values determined under the original assumptions.
In summary, this simple model based on the idea that R* decay can be represented as a double-exponential function in which phosphorylation proceeds independently of the rate of Arr1 binding is able to capture seemingly disparate results of response recovery in both dim and saturating flash regimes of our four mouse lines. A single set of three parameters (τk, τawt, τa+/−) can quantitatively account for all six major features of our recovery kinetic data, including (1) the difference in τrec and (2) the similarity in τD for RGS9-ox and Arr1+/−RGS9-ox responses, the similarity in both (3, 4) τrec and τD for WT and Arr1+/− responses, and (5, 6) the increase in Tsat for both Arr1+/−RGS9-ox and Arr1+/− saturating responses relative to RGS9-ox and WT saturating responses, respectively.
Discussion
Estimation of R* lifetime: the dependence on Arr1 expression
Overexpression of the RGS9 complex dramatically accelerates recovery of both dim and saturating flash responses, indicating that Gtα/PDE deactivation normally rate-limits recovery and setting an upper bound on the lifetime of R* (Krispel et al., 2006; Chen et al., 2010). The highest overexpression of RGS9 achieved to date indicates that in dark-adapted rods, R* deactivation proceeds with a time constant of ≤54 ms (Chen et al., 2010), and theoretical work suggests that it is probably <50 ms (Burns and Pugh, 2009). The results in this study further support the idea of a short R* lifetime: our data and analysis show that in normal rods, R* deactivation proceeds with a time constant equal to 36 ms.
Our analysis suggests that in wild-type rods the outer segment level of Arr1 is such that phosphorylation and Arr1 binding proceed at approximately the same rates, allowing R* deactivation to be well approximated by a single exponential. The similarity in these rates should help to make the pulse of R* activity more similar from trial to trial, which is thought to be important for the reproducibility of the single-photon response (Rieke and Baylor, 1998). A biochemically realistic mathematical model for reproducibility that incorporates faster R* deactivation will be necessary to understand the significance, or coincidence, of the similarity in these rates of phosphorylation and arrestin binding in normal rods. To date, the shortest R* lifetime that has been used in modeling reproducibility is 118 ms (Bisegna et al., 2008).
Our results directly contradict a recent study (Doan et al., 2009), which reported that R* deactivation rate-limits recovery, and that R* deactivation is slightly faster when Arr1 is underexpressed. Doan et al. (2009) proposed that their findings may have been unique to their recording conditions, which used Ames' medium rather than Locke's. However, we found that RGS9 overexpression dramatically accelerates response recovery more than twofold in Ames' medium (supplemental Fig. S2, available at www.jneurosci.org as supplemental material), similar to what has been reported in Locke's solution (Krispel et al., 2006; this present study) and in Eagle's medium (Chen et al., 2010). Thus, Gtα/PDE deactivation remains rate limiting even in Ames' medium. By extension, the conclusion of Doan et al. (2009) that R* deactivation is 22% faster in Arr1+/− rods is likewise refuted by the dramatic effect of RGS9-overexpression in Ames, and their competition model for R* deactivation, which is based on a long R* lifetime, cannot be correct. [Further discussion of Doan et al. (2009) is provided in the supplemental material, available at www.jneurosci.org.] In contrast, our results support a traditional biochemical scheme in which the rate of phosphorylation is independent of Arr1 concentration, and lowering Arr1 concentration slows R* deactivation slightly by reducing the rate of Arr1 binding.
The slowed rate of Arr1 binding in Arr1+/− rods can be used to estimate the concentration of Arr1 available to bind R* in dark-adapted mouse outer segments. Biochemical studies have indicated that the association rate constant for Arr1 and phosphorylated R* is ∼1 μm−1 · s−1 (Schleicher et al., 1989; Pulvermüller et al., 1997). In rods with reduced Arr1 expression, our calculated Arr1 binding rate of 15 s−1 (1/67 ms) corresponds to an effective OS Arr1 concentration of 15 μm in Arr1+/− rods. For wild-type rods with a binding rate of at least 28 s−1 (1/36 ms), the corresponding calculation yields an effective Arr1 concentration of at least 28 μm, which is close to previous estimates for endogenous OS Arr1 monomer in bovine rods (Gurevich et al., 2007).
Our conclusion that the rate of Arr1 binding changes in nearly direct proportion to a change in total OS Arr1 content is at odds with the emerging notion that the amount of free Arr1 available to bind R* is buffered through oligomerization (Gurevich et al., 2007; Hanson et al., 2007a; Hanson et al., 2007b). Dissociation constants for bovine Arr1 determined at room temperature for the formation of Arr1 dimers and tetramers predicts that the 1.9-fold reduction in Arr1 monomer concentration calculated above would be accompanied by a fourfold reduction in total Arr1 expression, rather than the 1.8-fold that we observe experimentally (supplemental Fig. S1, available at www.jneurosci.org as supplemental material). Our results suggest that the Kd for dimerization of mouse Arr1 at physiological temperatures must be significantly greater than that determined for bovine Arr1 (Hanson et al., 2007a), so that the amount of available Arr1 monomer, and thus the rate of Arr1 binding, does indeed vary as the total Arr1 content of the outer segment changes.
Implications for light-dependent movement of Arr1
The total Arr1 content in the outer segment changes dramatically with light exposure (for review, see Calvert et al., 2006). In mouse rods, the OS Arr1 concentration can vary as much as ∼10-fold between dark-adapted conditions and light exposures that activate ∼3% of the total rhodopsin over a span of 10 min (Strissel et al., 2006). Our results on dark-adapted rods can also be used to estimate the functional consequences that Arr1 translocation of this magnitude would have on R* lifetime. Under our simple model, the rate of Arr1 binding to phosphorylated R* would increase nearly in proportion to the increase in OS Arr1 content, predicting that τa would decrease from 36 ms to ∼4 ms. If the rate of phosphorylation is unaffected, the integrated PDE activity from a given flash response would decrease by only 24%. Thus, even large (10-fold) changes in Arr1 levels are predicted to produce only modest changes in flash responses. (Here we are focused only on R* deactivation, rather than any effect of Arr1 levels on amplification through competition with Gtα for R*.) Our calculation suggests that the time course with which R* activity decays is primarily determined by phosphorylation, because the phosphorylation rate determines Arr1 binding independently of Arr1 content.
Control of the single-photon response amplitude by Arr1 expression in RGS9-overexpressing rods
In addition to the noted effects on recovery kinetics, underexpression of Arr1 increased the SPR amplitude in the RGS9-ox background, but not the wild-type background (Table 1). A similar observation was also made in a recent study that showed that sensitivity was unchanged when R* lifetime was lengthened by underexpressing GRK1 in the wild-type background, but that it was substantially increased by GRK1 underexpression in the RGS9 overexpression background (Chen et al., 2010). We propose that this differential effect of R* lifetime in WT and RGS9-ox backgrounds stems from differences in the calcium-dependent regulation of cGMP synthesis, which strongly affects SPR amplitude (Burns et al., 2002). For example, if the dark PDE activity is reduced in rods that overexpress RGS9, then the dark calcium levels would be slightly elevated and the dark rate of cGMP synthesis would also be reduced. As a consequence, there would be less activation of guanylate cyclase in response to the change in calcium that accompanies the flash response in RGS9-ox rods, unmasking the lengthened R* lifetime associated with Arr1 underexpression. Conversely, in the WT background higher rates of cGMP synthesis during the light response dampen small increases or decreases in R* lifetime more strongly. This mechanism may explain why sensitivity is preserved in rods that overexpress GRK1 (Krispel et al., 2006; Whitcomb et al., 2009) or lack the GRK1 inhibitory protein, recoverin (Makino et al., 2004).
Estimation of the rate of rhodopsin phosphorylation in wild-type rods
Our double-exponential model suggests that in wild-type rods, phosphorylation by GRK1 initially decreases R* activity with an overall rate of ∼28 s−1 (1/36 ms). Importantly, the rate provided by this model does not address the number of phosphorylations that precede Arr1 binding, since the durations of each progressive GRK1 binding event and phosphate transfer leading to Arr1 quench are rolled into the aggregate time constant. While several electrophysiology studies have suggested that 3–6 phosphorylation sites are necessary for normal deactivation of R* (Mendez et al., 2000; Doan et al., 2006), biochemical studies show that two of these sites need to be phosphorylated to increase the affinity of Arr1 appreciably and that a minimum of three phosphorylations are required for high-affinity binding (Vishnivetskiy et al., 2007). Perhaps the extra phosphorylation sites at the flexible, relatively unstructured C terminus of rhodopsin (Palczewski et al., 2000; Park et al., 2008) increase the rate of phosphorylation by increasing the local substrate for GRK1. Faster phosphorylation associated with an excess of possible phosphorylation sites would lead to more rapid Arr1 binding and consequently faster overall R* deactivation. Testing this idea would further tease apart the relative rates of phosphorylation and arrestin binding, which is essential for understanding the balance between signal amplification and rapid, reliable recovery in rods.
Footnotes
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This work was supported by National Eye Institute Grants EY014047 (R01 to M.E.B.) and EY015387 (Training Program in Vision Science in partial support of O.P.G.). We thank E. N. Pugh Jr for critically reading this manuscript.
- Correspondence should be addressed to Marie E. Burns, Center for Neuroscience, University of California, Davis, 1544 Newton Court, Davis, CA 95618. meburns{at}ucdavis.edu