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The Journal of Neuroscience, February 25, 2004, 24(8):1936-1940; doi:10.1523/JNEUROSCI.4554-03.2004
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Loss of Kv3.1 Tonotopicity and Alterations in cAMP Response Element-Binding Protein Signaling in Central Auditory Neurons of Hearing Impaired Mice
Christian A. A. von Hehn, * Arin Bhattacharjee, * andLeonard K. Kaczmarek Department of Pharmacology, Yale University School of Medicine, New Haven, Connecticut, 06520
Abstract
Top
Abstract
Introduction
The promoter for the kv3.1 potassium channel gene is regulated by a Ca2+-cAMP responsive element, which binds the transcription factor cAMP response element-binding protein (CREB). Kv3.1 is expressed in a tonotopic gradient within the medial nucleus of the trapezoid body (MNTB) of the auditory brainstem, where Kv3.1 levels are highest at the medial end, which corresponds to high auditory frequencies. We have compared the levels of Kv3.1, CREB, and the phosphorylated form of CREB (pCREB) in a mouse strain that maintains good hearing throughout life, CBA/J (CBA), with one that suffers early cochlear hair cell loss, C57BL/6 (BL/6). A gradient of Kv3.1 immunoreactivity in the MNTB was detected in both young (6 week) and older (8 month) CBA mice. Although no gradient of CREB was detected, pCREB-immunopositive cells were grouped together in distinct clusters along the tonotopic axis. The same pattern of Kv3.1, CREB, and pCREB localization was also found in young BL/6 mice at a time (6 weeks) when hearing is normal. In contrast, at 8 months, when hearing is impaired, the gradient of Kv3.1 was abolished. Moreover, in the older BL/6 mice there was a decrease in CREB expression along the tonotopic axis, and the pattern of pCREB labeling appeared random, with no discrete clusters of pCREB-positive cells along the tonotopic axis. Our findings are consistent with the hypothesis that ongoing activity in auditory brainstem neurons is necessary for the maintenance of Kv3.1 tonotopicity through the CREB pathway.
Key words: auditory; Kv3.1; MNTB; CREB; tonotopicity; presbyacusis
Introduction
Age-related hearing-loss (presbyacusis) is the most common cause of adult auditory deficiency in the United States. Although progressive loss of hair cell function is a main pathogenic factor, it is not clear whether presbyacusis involves only the dysfunction of sensory hair cells or whether there are also resultant changes in auditory neurons (Boettcher, 2002; Seidman et al., 2002
The first integration of binaural inputs occurs in the superior olivary complex (SOC). Within the SOC, the medial nucleus of the trapezoid body (MNTB) functions as a fast sign-inverting relay station. Precisely timed inhibitory input from the MNTB to the medial and lateral superior olive is required for comparison of interaural time and level differences and therefore for sound localization (Grothe, 2003
The potassium channel Kv3.1 is generally expressed in neurons that are capable of firing action potentials at high rates. It is expressed at particularly high levels in the auditory brainstem, including the MNTB (Luneau et al., 1991
Kv3.1 is the only neuronal potassium channel for which transcription is known to be regulated by the CA2+-cAMP-responsive element binding protein (CREB) transcription factor (Gan et al., 1996
In this study we have examined the localization of Kv3.1, CREB, and the phosphorylated form of CREB (pCREB) in normal-hearing CBA mice at both 6 weeks and 8 months of age, and in BL/6 mice at the same stages. At 6 weeks the hearing of BL/6 mice is apparently normal, whereas at 8 months hearing is clearly impaired (Parham and Willott, 1988
Materials and Methods
Six-week- and 8-month-old CBA/J and C57BL/6 and 8-month-old DBA/2J male mice were tested for auditory impairment with a startle test (Parham and Willott, 1988All pictures were taken on an Olympus BX60 microscope by using a SPOT RT digital camera (Diagnostic Instruments, Sterling Heights, MI). Optical density (OD) and integrated optical density (IOD) were measured using ImagePro Plus software (Media Cybernetics, Silver Spring, MD). For CREB and pCREB, the software automatically determined nuclear staining. For Kv3.1, the outline of each cell was drawn manually, and the maximal optical density was measured. Where appropriate, the relative optical density was calculated by normalizing all obtained optical densities on a section to the highest density on the section.
Results
In coronal sections of the brainstem, neurons within the MNTB are organized tonotopically, with low-frequency neurons located laterally and high-frequency neurons located medially (Sommer et al., 1993
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Figure 1. Quantification of tonotopic gradient of Kv3.1 in the MNTB. Left, Coronal sections of the MNTB of CBAs and BL/6 mice (6 weeks and 8 months). Right, Four individual sections for each strain and age group were divided in five equal segments from lateral to medial. The mean Kv3.1 OD of all cells within each segment was measured and normalized to the darkest cell in each section. The gradient of Kv3.1 immunoreactivity is clear in all sections (p < 0.05), except for old BL/6 mice. The data are representative of four animals for each age group and strain. Lines through data show results of regression analysis; R values for sections from young CBA: 0.9142, 0.90744, 0.94096, 0.96983; R values for sections from old CBA: 0.96237, 0.96336, 0.96249, 0.93388; R values for sections from young BL/6: 0.97647, 0.97202, 0.98277, 0.82361; R values for sections from old BL/6: 0.77473, -0.43453, -0.05161, -0.7349. Scale bar, 250 µm. A tonotopic gradient in Kv3.1 immunoreactivity was also absent in 8-month-old DBA/2J mice, which are hearing impaired (data not shown).
The kv3.1 gene is regulated by CREB and by depolarization (Gan et al., 1996
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Figure 2. CREB immunoreactivity in the MNTB and the cerebellum. A, Examples of four MNTB sections from each strain and age group. B, The MNTB was divided into six equal segments from lateral to medial. The IOD was measured for individual cells of each section. Lines through data show results of regression analysis. Comparing the two strains, from lateral to medial, no tonotopic increase of CREB immunoreactivity was found. Slopes of both lines did not significantly differ from zero; R value for old CBA: -0.77121; R value for old BL/6 -0.89616. C, There was a 50% decrease, however, of total CREB immunoreactivity in the MNTB of BL/6 compared with CBA. D, Using the same sections containing the MNTB, we also examined cerebellar Purkinje cells of both strains; there was no significant difference in IOD between the two strains. n = 5 for both strains; error bars represent SEM; *p < 0.05 determined by unpaired t test. Scale bar, 250 µm.
As a control for this difference in CREB staining between the 8-month-old BL/6 and CBA mice, we also analyzed CREB staining in the cerebella of the two species. Such staining would not be expected to be influenced by changes in auditory function. In coronal sections of the mouse brainstem, the MNTB and parts of the cerebellum are located on the same slice (Franklin and Paxinos, 1997Because CREB is only active as a transcription factor when it is phosphorylated, we investigated the distribution of activated pCREB by staining sections of the MNTB with a CREB-Ser133 phospho-specific antibody. Interestingly, in mice with intact audition (6-week- and 8-month-old CBA, 6-week-old BL/6), we found a pattern that differed from mouse to mouse. Like CREB itself, the staining for pCREB was confined to the nucleus. Nevertheless, only subsets of neurons were labeled with the pCREB antibody, whereas others appeared devoid of labeling. Strikingly, labeled neurons were always grouped into discrete clusters, which were distributed along the tonotopic axis in each section (Fig. 3).
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Figure 3. pCREB immunoreactivity in MNTB of old CBAs. A, Example of a coronal MNTB section of an 8-month-old CBA stained for pCREB. Inset, Density distribution histogram demonstrating the bimodality of pCREB staining. B, Optical densities over nuclei from all cells within four individual MNTBs were counted across the medial-lateral axis. Cells with a relative pCREB OD >0.5 were assigned 1; cells with a relative pCREB OD <0.4 were assigned 0. The data are representative of five animals for each age group. Scale bar, 250 µm.
To quantify the clustering along the tonotopic axis, we first established that pCREB labeling was binary, i.e., that a given neuron could be uniquely assigned as pCREB positive or pCREB negative. The distribution of densities detected in neurons stained for pCREB was found to be clearly bimodal (Figs. 3A, insert, 4A, insert), with the peak of the lower density corresponding to unstained nuclei. As a result, it is possible to give each neuron a score of "1" for a stained nucleus and "0" for an unstained nucleus (Figs. 3, 4). Figure 3 illustrates the clustering of pCREB staining along the medial to lateral axis in the form of a "bar code" for four different MNTBs of normal-hearing old CBAs. To quantify the pattern of clustering of pCREB staining we used the Runs test for detecting non-randomness and obtained p values (<0.0001) for all sections, indicating that these sequences are significantly different from a random distribution of staining.
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Figure 4. pCREB immunoreactivity in MNTB of old BL/6 mice. A, Example of a coronal MNTB section of an 8-month-old BL/6 stained for pCREB. Inset, Density distribution histogram demonstrating the bimodality of pCREB staining. B, The optical densities over nuclei from all cells within four individual MNTBs were counted across the medial-lateral axis. Cells with a relative pCREB OD >0.5 were assigned 1; cells with a relative pCREB OD <0.4 were assigned 0. The data are representative of four animals for each age group. Scale bar, 250 µm. A similar pattern of pCREB immunoreactivity was found in hearing-impaired DBA/2J mice (data not shown).
In contrast to the normal-hearing animals, pCREB labeling in the hearing-impaired BL/6 and DBA/2J mice provided no evidence of clusters along the medial-lateral axis. Instead, staining appeared to be randomly distributed over the tonotopic axis of the MNTB, as revealed by a comparison of the barcodes for these animals (Fig. 4). Defining a cluster as one or more adjacent stained cells, we found that the pattern of pCREB staining of hearing-impaired animals was significantly different from that of the hearing mice (mean cluster size CBA: 9.13 ± 2.98 (SEM) cells; mean cluster size BL/6: 1.77 ± 0.08 cells; p < 0.0001).As shown here for the MNTB, pCREB labeling in the VCN of normal-hearing CBA and 6-week-old BL/6 mice also revealed discrete clusters of staining, and again in 8-month-old BL/6 mice, pCREB staining appeared to be distributed randomly in the VCN (data not shown).
Discussion
We have found that a tonotopic gradient of Kv3.1 expression in the MNTB is present in young BL/6 mice when their hearing is normal but that the gradient is lost later in life when hearing is impaired. The loss of the gradient is accompanied by a decrease in CREB and a change in the distribution of pCREB, the activated, phosphorylated transcription factor. In particular, the deficit in hearing is associated with the loss of discrete clusters of pCREB-positive cells along the tonotopic axis. In contrast, in the CBA mouse species, which maintains good hearing throughout its life, the tonotopic gradient of Kv3.1 and the localization of pCREB to discrete cell clusters in the MNTB are maintained through adulthood. Although loss of sensory input is associated with a small loss of neurons in some central nuclei (Willott and Bross, 1996The genetic basis for the loss of cochlear hair cells in BL/6 mice is thought to be caused by a genetic defect of the cdh23 gene (Noben-Trauth et al., 2003
Because the transcription of the Kv3.1 is regulated by CREB (Gan et al., 1996
A decrease in Kv3.1 levels would be expected to compromise the ability of auditory neurons to maintain temporal precision at high rates of stimulation. In brain slice preparations, MNTB neurons lock their action potentials to imposed stimuli at frequencies of up to 600 Hz (von Gersdorff and Borst, 2002
We have found that pCREB-immunopositive cells are distributed in clusters of cells within relatively broad frequency bands along the tonotopic axis of the MNTB. One of the most common stimuli leading to CREB phosphorylation in neurons is Ca2+ influx through voltage-dependent channels activated by neuronal firing, and even short bursts of action potentials have been found to activate CREB phosphorylation (Bonni et al., 1995
Footnotes
Received Oct 7, 2003; revised January 11, 2004; accepted January 11, 2004.This work was supported by National Institutes of Health Grants DC-01919 and NS42202 and by the American Federation for Aging Research. We thank U. Schulz and J. Hedderich for statistical advice.
Correspondence should be addressed to Leonard K. Kaczmarek, Department of Pharmacology, Yale University School of Medicine, 333 Cedar Street, New Haven, CT 06520. E-mail: leonard.kaczmarek{at}yale.edu.
Copyright © 2004 Society for Neuroscience 0270-6474/04/241936-05$15.00/0
* C.A.A.H. and A.B. contributed equally to this work.
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