This video illustrates a method, using a clinical 3 T scanner, for contrast-enhanced MR imaging of the naïve mouse visual projection and for repetitive and longitudinal in vivo studies of optic nerve degeneration associated with acute optic nerve crush injury and chronic optic nerve degeneration in knock-out mice (p50KO).
The rodent visual system encompasses retinal ganglion cells and their axons that form the optic nerve to enter thalamic and midbrain centers, and postsynaptic projections to the visual cortex. Based on its distinct anatomical structure and convenient accessibility, it has become the favored structure for studies on neuronal survival, axonal regeneration, and synaptic plasticity. Recent advancements in MR imaging have enabled the in vivo visualization of the retino-tectal part of this projection using manganese mediated contrast enhancement (MEMRI). Here, we present a MEMRI protocol for illustration of the visual projection in mice, by which resolutions of (200 µm)3 can be achieved using common 3 Tesla scanners. We demonstrate how intravitreal injection of a single dosage of 15 nmol MnCl2 leads to a saturated enhancement of the intact projection within 24 hr. With exception of the retina, changes in signal intensity are independent of coincided visual stimulation or physiological aging. We further apply this technique to longitudinally monitor axonal degeneration in response to acute optic nerve injury, a paradigm by which Mn2+ transport completely arrests at the lesion site. Conversely, active Mn2+ transport is quantitatively proportionate to the viability, number, and electrical activity of axon fibers. For such an analysis, we exemplify Mn2+ transport kinetics along the visual path in a transgenic mouse model (NF-κB p50KO) displaying spontaneous atrophy of sensory, including visual, projections. In these mice, MEMRI indicates reduced but not delayed Mn2+ transport as compared to wild type mice, thus revealing signs of structural and/or functional impairments by NF-κB mutations.
In summary, MEMRI conveniently bridges in vivo assays and post mortem histology for the characterization of nerve fiber integrity and activity. It is highly useful for longitudinal studies on axonal degeneration and regeneration, and investigations of mutant mice for genuine or inducible phenotypes.
Based on its favorable neuro-anatomical structure the rodent visual system offers unique possibilities to evaluate pharmacological compounds and their capability to mediate neuroprotection1 or pro-regenerative effects2,3. Moreover, it allows studies on the functional and neuro-anatomical characteristics of mouse mutants, as recently exemplified for mice lacking the presynaptic scaffolding protein Bassoon4. Furthermore, a broad spectrum of supplementary tools affords additional featuring of retinal ganglion cell (RGC) and RGC axon numbers as well as RGC activity, e.g., by electroretinography and behavioral tests, and the determination of cortical rearrangements by optical imaging of intrinsic signals. The latest technical developments in laser microscopy enable the in situ visualization of RGC regeneration by deep tissue fluorescence imaging in whole mount specimens of optic nerve (ON) and brain. In this histological approach, tetrahydrofuran based tissue clearing in combination with light sheet fluorescence microscopy permits the resolution of single fibers that re-enter into the deafferented ON and optic tract 5. While such techniques might be superior in resolution and determination of growth patterns, they do not enable repetitive and longitudinal analyses of individual growth events, which are particularly desired to assess the process of long term regeneration.
Contrast-enhanced MRI has been employed for the minimal invasive visualization of the retino-tectal projection in mice and rats6,7. This can be achieved by direct intraocular delivery of paramagnetic ions (e.g., Mn2+) to retinal cells. As a calcium analog, Mn2+ is incorporated into RGC somata via voltage-gated calcium channels and actively transported along the axonal cytoskeleton of the intact ON and optic tract. While it accumulates in brain nuclei of the visual projection, i.e. the lateral geniculate nucleus (LGN) and superior colliculus (SC), transsynaptic propagation into the primary visual cortex appears negligible8,9, although it may occur10,11. Under MR sequencing, paramagnetic Mn2+ augments MR contrast mainly by shortening T1 spin-lattice relaxation time12. Such Mn2+ enhanced MRI (MEMRI) has been successfully applied in various neuro-anatomical and functional studies of rats, including the assessment of axonal regeneration and degeneration after ON injury13,14, the precise anatomical mapping of the retino-tectal projection15, as well as the determination of axonal transport characteristics after pharmacological treatment16. Recent refinements in the dosage, toxicity, and kinetics of neuronal Mn2+ uptake and transport, as well as improved MRI protocols have extended its application to studies on transgenic mice9 using 3 Tesla scanners commonly used in clinical practice17.
Here, we present a MEMRI protocol suitable for longitudinal in vivo imaging of the mouse retino-tectal projection and exemplify its applicability by assessing Mn2+ dependent signal enhancement under naïve and various neurodegeneration conditions. Our protocol places specific emphasis on MR data acquisition in a moderate 3 T magnetic field that is generally more accessible than dedicated animal scanners. In naïve mice, we illustrate how tract-specific signal intensity can be substantially and reproducibly become increased after intravitreal (ivit) Mn2+ application. Quantitatively, Mn2+ propagation along the visual projection occurs independently of the normal aging process (measured between 3 and 26 month old mice) and augmentation is refractory to visual stimulation and adaptation to darkness. In contrast, Mn2+ enrichment in thalamic and midbrain centers is diminished following acute ON crush injury18 as well as in nfkb1 knock-out mice (p50KO) suffering from spontaneous apoptotic RGC death and ON degeneration19. Thus, in expansion to conventional histological analysis, longitudinal MEMRI analysis of individual animals enables profiling of unique kinetics of neurodegenerative processes. This should prove useful for studies on neuroprotection and axonal regeneration associated with pharmacological or genetic interventions.
All animal interventions are performed in accordance with the European Convention for Animal Care and Use of Laboratory Animals and the ARVO Statement for the Use of Animals in Ophthalmic and Vision Research. All experiments are approved by the local ethics committee. The procedure of ON injury in mice is described elsewhere9.
1. Intravitreal Manganese Injection
2. Animal Preparation for MRI
3. MRI Protocol
4. MRI Data Analysis
5. Mn2+ Autometallography (TIMM Staining)
6. Statistical Analysis
Perform statistical analyses using the Student’s t-test for single comparisons, followed by post hoc ANOVA. Data are presented as mean ± standard error. Individual N numbers are given separately for each experiment. Results reaching P ≤ 0.05 are considered statistically significant (P ≤ 0.05, *; P ≤ 0.01, **; P ≤ 0.001, ***).
The ability of this imaging technique to accurately assess the vitality and functionality of the visual projection relies upon precise application of a nontoxic Mn2+ dosage to the vitreous body and its uptake by RGCs. This major assumption is tested in Figure 1, where layer specific Mn2+ uptake is demonstrated by autometallography (TIMM staining)21. Retina sections were analyzed at 24 hr after ivit application of either 15 nmol or 150 nmol Mn2+, or PBS as control. At this time point, the Mn2+ injected retinae show maximum signal enhancement in T1 weighted MRI (N = 3; dotted lines), whereas the PBS injected retina is not enhanced in signal (N = 3; dotted line) (Figure 1, left panel). Note the hyperintensive signal enhancement in the 150 nmol injected eye. In contrast, nonenhanced brain areas (asterisks) show similar background signal intensities for all conditions (green color). Ivit Mn2+ application increases overall TIMM staining particularly in the RGC layer and nerve fiber layer (NFL) (Figure 1, magnified insets in middle panel), which are confirmed by investigation of individual RGC somata following H & E co-labeling (right panel).
For in vivo imaging of the mouse retino-tectal projection, it is critical to select a special mouse MEMRI protocol where the operational parameters together with the equipment, as illustrated in Figure 2, are adapted to analyze mice in a 3 T field. Applying such a scanner setup, our earlier work revealed that for CNS image resolution a rat head coil is superior to a dedicated mouse whole body coil17. To fix the murine head and to properly adjust its position within the rat coil, we use a cradle and a conical tube with bite bar made of plastic, both of which are downscaled to meet the body dimensions of mice (Figures 2A,B). When images are acquired on a transversal T1 weighted matrix implementing 3D gradient echo sequences, the generation of high-resolution images of (200 µm)3 within 35 min of acquisition time can be expected. We strongly recommend the constant monitoring of vital functions during the scan. Adjustment of anesthesia together with postimaging oxygenation and body temperature control significantly accelerates recovery time and guarantees survival rates of about 100%. Such technical precautions are essential to ensure that the whole cohort will sustain longitudinal and repetitive MRI.
In any study, only a nontoxic Mn2+ dosage of 15 nmol should be used for ivit application9, which is sufficient to prominently enhance CNRs in the retina, ON, and optic tract up to the presynaptic intracerebral LGN and SC. CNR values are best calculated from 200 µm thick transversal slices obtained from original MRI data sets by reslicing the original isotropic 3D volume. Figure 3A shows an example of precise CNR determination for the enhanced LGN, where three regions of interest are selected in each image for (1) signal-enhanced area (SIMEMRI), (2) non-affine brain tissue (SIbackgr), and (3) background noise (SDN). The expectable spatial signal enhancement quantified along the entirety of a single visual projection is presented in Figure 3B. Note the strong gradual increase of signal enhancement in retinal sections along the dorsoventral plane, which peaks at the optic nerve head. Additionally, note the lack of a relevant transsynaptic Mn2+ propagation into cortical layers under the applied experimental conditions (signal drop in the visual cortex). MIPs are highly illustrative to visualize the 3D positioning of the retino-tectal projection in toto (Movie 1). Accumulation of Mn2+ along the visual projection is determined by the kinetics of intracellular uptake into RGCs through voltage dependent Ca2+ channels and its fast axonal transport, as well as by the relatively low clearance from the target tissue13. According to our previous kinetic studies, Mn2+ dependent signal enhancement can be detected as early as 6 hr after injection. It further peaks at 24 hr and decreases back to baseline levels within 120 hr post-injection9. Therefore, to achieve optimum results, MEMRI should be performed 24 hr after injection, which represents half of the enhancement time required for rats13.
Having outlined the principle for contrast enhancement of the visual projection by MEMRI, we further communicate the influences of two parameters – light condition and animal age – that may affect quantitative measurements:
(1) To test for stimulus-dependent accumulation of Mn2+ in midbrain centers, mice were kept either under light-stimulated conditions achieved by flashlight exposure of a defined frequency (5 Hz) and light intensity (3 W LED) or in complete darkness prior to the scan and during 24 hr of Mn2+ exposure. Quantitative analysis of the CNR 24 hr after ivit Mn2+ application reveals a significant increase in the signal intensity of dark-adapted retinae compared to light-stimulated conditions (66.29 ± 3.07 vs. 54.56 ± 3.08, P ≤ 0.05, N = 7/8; Figure 3C). Given the gradient in signal enhancement between the peripheral retina and the optic nerve head (see Figure 3B), we assured to always analyze corresponding retinal sections within all experimental groups. Image analysis along the ventrodorsal plane revealed, as expected, that absolute CNR values are going down in both conditions. Importantly, the relative signal difference between dark and light adapted retinae remains persistent (data not shown). However, signal enhancement in the projection areas of LGN (26.97 ± 1.78 vs. 26.58 ± 1.05, P = 0.9, N = 7–2) and SC (25.09 ± 1.24 vs. 26.81 ± 1.55, P = 0.4, N = 7/8) is indistinguishable between light and dark conditioning environments (Figure 3C). This assay demonstrates that uptake of Mn2+ into retinal layers is sensitive to light exposure, whereas its propagation along the retino-tectal projection and accumulation in target areas is not influenced by coincident visual stimulation. Alternatively, the signal sensitivity of the 3 T scanner might be below the detection threshold for signal variation in the LGN or SC.
(2) To explore implications of the animal’s age on MEMRI related signal enhancement of the visual projection, we analyzed mice between 3 and 26 months of age. CNR values in the LGN of 3 months old mice (23.49 ± 1.36, N = 12) do not differ from the signal intensity measured in mice aged 7 months (23.90 ± 0.81; P = 0.79, N = 16), 13 months (23.35 ± 1.29, P = 0.94, N = 10) or 26 months (25.10 ± 2.29, P = 0.53, N = 6; Figure 3D). Likewise, the signal intensity in the SC is unchanged between 3 months (19.01 ± 1.20) and 26 months of age (16.92 ± 2.18, P = 0.37; Figure 3D). Although a slight increase is evident in the CNR values of 26 month old retinae (38.49 ± 3.25), this increase does not reach significance when compared throughout all the groups (P > 0.05). These experiments indicate that signal enhancement in cerebral target areas of the visual projection is unaffected by visual stimulation and physiological aging.
Next, we demonstrate the sensitivity of MEMRI to detect structural alterations of the visual projection caused by acute and chronic axonopathy. To explore this, a model of Wallerian degeneration induced by traumatic ON injury18 as well as an animal model displaying precocious, spontaneous degeneration of sensory projections including the visual pathway19 were employed:
(1) Traumatic axonopathy induced by ON crush injury causes the breakage of axona fascicles. Consequently, retino-tectal transport of Mn2+ along the axonal cytoskeleton will be completely and sustainably blocked, as visualized by complete loss of Mn2+ enhanced signal in the LGN and SC analyzed one day (not shown), one week (Figure 4A, dotted lines), and 4 weeks (not shown) post injury. To clearly demonstrate the neuroanatomical and consecutive MR features of ON injury and to dissect them from the naïve state, the lesion was inflicted only unilaterally. This results in unaltered Mn2+ transport on the control side in contrast to tracer interruption on the side of the intervention. Analysis of CNR values in the deafferented areas confirms the complete absence of signal enhancement (not shown). This experiment further demonstrates that MEMRI is highly sensitive in detecting the location and severity of a lesion site by longitudinal assessment of the signal intensity along the projection before and after injury (Figure 4B). While the signal intensity along the ON before injury constantly stays above the background signal, there is a temporo-spatial drop in signal intensity to the background level one day after ON injury.
(2) Our earlier work demonstrated that Mn2+ dependent signal enhancement in the LGN is reduced in 10 months old mice lacking the NF-κB subunit p50 when measured 24 hr after injection9. Detecting this with a high consistence, we assumed an overall impairment in retino-tectal Mn2+ transport, possibly caused by reduced numbers of RGCs and related ON neuropathy in aging p50KO mice19. Alternatively, the reduced signal enhancement might be associated with a delayed neuronal uptake and propagation of Mn2+ from the vitreous body and along the pathological projection. The latter possibility can be explored by performing repetitive MR scans after a single application of 15 nmol Mn2+ and studying the kinetics of signal enhancement in the retina and LGN at early (8 and 24 hr) and late (48 and 72 hr) time points. In wild type and p50KO mice, retinal signal enhancement peaks at 8 hr at almost identical enhancement rates (43.52 ± 3.24 and 40.72 ± 2.79; P = 0.6, N = 3–6; Figure 4C, left). While signal enhancement remains high in wild types at 24 hr post injection, it declines in p50KO mice (43.38 ± 2.18 vs. 32.89 ± 1.54; P ≤ 0.01, N = 5–8). During later phases (48 and 72 hr), signal enhancement decreases in both groups (with consistently lower CNR values in knock-out mice), thus excluding a delayed retinal Mn2+ uptake and propagation in p50KO mice. Corresponding results in the LGN of p50KO mice confirm this notion. Although the CNR is significantly lower between 8 and 48 hr post-injection (P ≤ 0.05, N = 5–9), the kinetics of signal attenuation in p50KO mice corresponds to that in wild type mice (Figure 4C, right). Thus, the reduced temporo-spatial signal enhancement of the retino-tectal projection is due to reduced axon numbers originating from a limited RGC population rather than impaired transport kinetics. We propose MEMRI to be a valuable tool to screen genetic mouse mutants for projectional impairments in the CNS.
Figure 1. TIMM staining of Mn2+ uptake in RGCs. Representative heat-map images of T1 weighted MRI (MRI T1) show signal enhancement of the lens and the whole retinal circumference (dotted line) 24 hr after ivit application of 15 nmol, and hyper-intensive signal enhancement after application of 150 nmol Mn2+ (left). Warm colors represent higher signal values than cold colors. Scale bar: 1 mm. Middle/right: Mn2+ uptake by RGCs after ivit injection of MnCl2 as detected by silver precipitation using TIMM staining (black color). PBS-treated control retina sections demonstrate rather weak staining and diffuse differentiation of the RGC layer (RGC) (top; N = 3). High magnification does not allow discrimination of individual cells (magnified insets). Ivit MnCl2 application differentially increases overall silver staining across retinal layers, with a prominent silver precipitation particularly in the nerve fiber layer (NFL), RGC layer, and inner nuclear layer (INL; middle and bottom, magnified insets; N = 3). Colabeling of TIMM with H & E staining further confirms such layer specific Mn2+ accumulation (right panel). Scale bar, overview: 50 µm, magnification: 25 µm. IPL, inner plexiform layer; OPL, outer plexiform layer; ONL, outer nuclear layer; RPE, retinal pigment epithelium.
Figure 2. Photographs showing MRI equipment specifically for mouse MEMR image acquisition on a clinical 3T scanner. A) shows the custom-made mouse cradle with bite bar head fixation and the sensor for respiratory monitoring (white pad, blue tube). B) shows the positioned and fixed mouse in the cradle. The tubes to the left supply the anesthetic gas. C) exemplifies the positioning of the mouse head and cradle inside the linearly polarized Litz coil operating in transmit and receive mode. D) shows the coil platform in front of the shielding tube and the clinical 3 T scanner. The copper coated tube provides additional shielding from noise and blocks the MRI signal from the hot water based heating mat (black wrapping around the tube). E) visualizes the complete set-up of the animal coil within the pore of the 3 T scanner just prior to positioning the animal head precisely at the isocenter inside the scanner.
Figure 3. MEMRI of the naïve retino-tectal projection under various light and age conditions. A) Illustration of region of interest (ROI) mapping in enhanced LGN and background tissue on a transversal MRI recording (left). LGN specific signal enhancement is illustrated by heat map presentation (right). 1 and 1’, left and right LGN; 2 and 2’, background tissue; 3, noise; P, posterior; R, right. Scale bar: 100 µm. B) Spatial mapping of signal enhancement along a single retino-tectal projection as determined from originally acquired transversal MR image slices by MEMRI. Filled squares, Mn2+ dependent signal enhancement; open triangles, background signal. R, retina; ON, optic nerve; OT, optic tract; LGN, lateral geniculate nucleus; SC, superior colliculus; VC, visual cortex. Slice thickness, 200 µm. C) Light stimulation significantly reduces retinal signal enhancement. Enhancement in the LGN and SC is independent of visual stimulation. Filled circles, dark-adaptation; open circles, light adaptation. D) Signal enhancement is independent of increasing age between 3 and 26 months.
Figure 4. MEMRI of the retino-tectal projection under neurodegenerative conditions. A) MEMRI of bilaterally ivit injected mice performed one week after unilateral crush injury of the right ON. Multiplanar reconstructions of horizontal, coronal, and lateral views depict complete absence of signal enhancement in the LGN and SC for the injured hemisphere (dotted lines). c, contralateral hemisphere; i, ipsilateral hemisphere. Scale bar: 1 mm. B) MIP images and longitudinal MRI analysis of the spatial signal enhancement along the ON before and one day after injury. R, retina; ON, optic nerve; arrow, lesion site. Scale bar: 0.5 mm. C) Kinetics of signal enhancement under chronic neurodegeneration of the visual projection in p50KO mice. Early (8 hr) uptake of Mn2+ into retinal cells is not affected, but is already reduced in the LGN of p50KO mice. Repetitive MR imaging at 24, 48, and (only for retina) at 72 hr shows sustained signal reduction, but similar kinetics of Mn2+ transport and accumulation in the retina and LGN of p50KO mice.
Movie 1: Animated, 3D heat-map presentation of the in situ contrast-enhanced retino-tectal projection. MR imaging was performed 24 hr after bilateral ivit injection of 15 nmol MnCl2. Data are presented in the MIP mode. Slice thickness, 200 µm. Please click here to view this video.
MEMRI of the visual system extends conventional neurobiological techniques for assessing functionality under naïve and pathological conditions. Apart from providing a unique insight into the integrity of an isolated CNS fiber tract, MEMRI can be easily supplemented with behavioral tests, e.g., optometry and visually based water tasks, to investigate the immediate consequences of a given paradigm for visual perception. It also links electrophysiological and histological investigations with functional visual characterization in vivo. The technique is highly reliable and reproducible with minor interindividual variances within identical groups (see error bars in Figures 3, 4). Intriguingly, at a dosage of 15 nmol, Mn2+ uptake and axonal transport are saturated processes, so that signal enhancement reaches a plateau which cannot be elevated by additional Mn2+ supply9. From a practical point of view, such a dose response characteristic minimizes, at least to some degree, injection associated variations in signal enhancement. Notably, the presented data on dosage and kinetics of Mn2+ signal enhancement are specific for mice and distinct from those in rats, which require an approximately 10-20x higher Mn2+ dosage and increased latency (36 hr) to achieve optimal contrast enhancement13,23. Additionally, enhancement along the visual projection remains consistent between an animal age of 3 and 26 months. This finding is in line with visual tests performed on aging mice and the fact that C57/B6 mice maintain normal visual activity up to 2 years of age24. Although we did not analyze individual mice longitudinally in the aging study, previous results clearly demonstrate the safety of repetitively administered Mn2+ dosages of 15 nmol for visual maintenance9, which might be desired in longitudinal aging studies.
In accordance with the notion that Mn2+ is incorporated into RGCs, we show Mn2+ uptake into their somata by TIMM staining which relies on silver precipitation of free metal ions, as applied by Angenstein et al. for intracerebral Mn2+ detection following its systemic application22. Previously, intracerebral Mn2+ distribution was detected by autoradiography of 54Mn2+ isotope to delineate neuronal circuits of the rat CNS25, but not at the cellular level. Here, TIMM staining allows the attribution of Mn2+ uptake to distinct cell populations within the exposed retina, where we find prominent silver precipitation in the RGC and nerve fiber layers. It should be noted that the protocol applied shows improved detection by TIMM staining after application of a dosage of 150 nmol compared to 15 nmol Mn2+. Although Mn2+ uptake and its axonal transport are already saturated at 15 nmol, thus, conferring no additional CNR increase along the retino-tectal projection at higher dosages, excessive supplementation might increase the availability of free, protein unbound Mn2+ and thus render it accessible for silver precipitation. Future refinements in staining sensitivity will allow the correlation of MEMRI-based CNR values of specific CNS projections with the cellular location of Mn2+ enrichment within a defined histological region. Such a capability might also be useful for the characterization and quantification of Mn2+ distribution in other CNS regions outside the visual projection. Likewise, Mn2+ has been employed in a kainate toxicity model to visualize degeneration and regeneration of hippocampal mossy fibers26.
Mn2+ is taken up by voltage dependent calcium channels and is intracellularly distributed by active axonal transport, which can be blocked by colchicine treatment25,27. Visual stimulation experiments on rats receiving an intraperitoneal dosage of MnCl2 have revealed an increased signal enhancement in the inner and, in particular, outer retina28. Thereby, dark adaptation further raises signal intensities in the outer retinal layers compared to rats exposed to room light conditions only, thus indicating sensitivity of retinal Mn2+ uptake to visual stimulation28. Similarly, we find enhanced signal intensity in the retina of dark adapted mice compared to mice exposed to visual stimulation after ivit Mn2+ application. This might be related to the specific electrophysiological properties of the retina and the generation of a continuous dark current in photoreceptor cells. Since Ca2+ influx into outer segments of photoreceptors significantly contributes to the constitution of the dark current, their generation might be accompanied by enhanced co-uptake of Mn2+ into the photoreceptor cell layer under darkness. In contrast, light stimulation reduces the dark current and causes hyperpolarization of photoreceptor cells29. Thereby, overall Mn2+ uptake might be diminished under light conditions.
For reliable usage of MEMRI, it is important to clarify whether the more pronounced Mn2+ uptake into the dark-adapted retina alters signal enhancement along other parts of the visual projection or even its entire extension. Stimulation-dependent changes in MEMRI signal intensity of cerebral networks have been demonstrated for the acoustic system after intraperitoneal Mn2+ application30. In this study by Yu et al., rats were exposed to variable noise frequencies before the MR scans and T1 weighted signal enhancement of the inferior colliculi was subsequently investigated. Acoustic stimulation was found to significantly increase MEMRI signal intensities in a tonotopic representation, thus exemplifying the fMRI-like character of activity-dependent Mn2+ accumulation30. In contrast, in our experimental set up Mn2+ accumulation in the LGN and SC appears independent of visual stimulation. However, such differences in sensory brain mapping attempts might arise from the lower magnetic field and limited threshold of detection of our 3 T scanner in comparison to the high field 7 T scanner used by Yu et al30.
To date, it is not known to what extent biophysical parameters affect anterograde axonal transport of Mn2+ and how MEMRI might serve as an indicator for electrical activity. Nevertheless, it appears that Mn2+ transmission by RGCs occurs, at least in part, independently of light specific stimulation and electrical input received from bipolar cells. Alternatively, the net effect of electrical activity within the retino-tectal projection might be a result of electrical stimulation of dark-responsive ‘OFF-RGCs’ and light-responsive ‘ON-RGCs’. Such an interpretation is supported by the finding that Mn2+ transport along the retino-tectal projection is not impaired in mouse strains with poor vision, such as CBA mice that carry the rd1 mutation of the Pde6b gene causing retinal degeneration11. In a kinetic study on wild type sighted and CBA mice, comparable transportation rates were observed during the initial influx phase (at 2.5 hr post-injection) and for the final signal enhancement (at 24 hr) in the LGN and SC11.
Taken together, these observations support the notion that MEMRI, e.g., of the visual system as exemplified here, represents a valuable measure for structural integrity and metabolic stability rather than for electrical activity. Practically, the seemingly stable independence of signal enhancement in cerebral LGN and SC from light exposure allows for robust handling and housing of animals without special care concerning illumination. On the other hand, for MEMRI studies that focus on retinal signal enhancement, it is necessary to keep animals under tightly controlled light conditions prior to the scan.
Among the physiological parameters that affect Mn2+ axonal transport rates and subsequent MEMRI signal enhancement, stability of body temperature might be of particular importance. This is indicated by studies on intranasal Mn2+ for enhancement of primary olfactory projection targets in the brain, where enrichment was found to be significantly diminished at a temporary reduction of body temperature to 30 °C compared to signal enhancement under normal body temperature27. Therefore, body temperature should be monitored and adjusted prior to and during the MR scans not only to protect the animals' health, but also to normalize physiological parameters of Mn2+ propagation.
Since pathophysiological alterations and metabolic impairments affect the axonal transport efficacy of Mn2+, signal enhancement in projection centers, e.g., LGN and SC, can serve as a measure for the structural integrity and functional activity of this pathway. Here, we present two different conditions of ON degeneration and illustrate that Mn2+ propagation and enrichment in thalamic and midbrain centers varies as a function of axonal integrity. Acute ON injury results in a total signal loss immediately after injury, which does not recover within 4 weeks due to the lack of relevant axonal regeneration, whilst slow axonal degeneration in the p50KO mutant is reflected by reduced CNR values in the LGN. Given the possibility of longitudinal imaging, this application of MEMRI might be valuable for monitoring postlesional growth responses of the ON and allow for the investigation of proregenerative genetic or pharmacological interventions to RGCs.
Additionally, we present MEMRI as a highly sensitive method to detect gradual impairments in signal enhancement that are associated with chronic axonal degeneration processes. The transcription factor NF-κB is involved in neuronal maintenance and mice with deletion of the p50 subunit of NF-κB display age-dependent neuronal cell loss and axonal degeneration within the visual system19. In addition to histological and electron microscopic analyses, MEMRI of the retino-tectal projection is able to identify phenotypic alterations in these mice. By acquisition of serial T1 weighted MR images following ivit Mn2+ application, we distinguished an overall reduced from a simply delayed Mn2+ transport along the visual pathway in these p50KO mice. Thereby, repetitive data acquisition by MEMRI after a single Mn2+ application enables the definition of axonal transport kinetics and neurophysiological alterations in the invaluable pool of available genetically modified mice. Currently, several modifications of MEMRI are under investigation aiming to make this technique safe for diagnostic applications in humans. A promising approach of high clinical relevance, which constitutes an alternative to ivit injection, is the delivery of Mn2+ as eye drops. Thereby, topical administration of 1 M MnCl2 yielded a significant signal enhancement by 20% in the SC when images were acquired on a 4.7 T animal scanner31. The method was able to detect extensive ON degeneration following retinal ischemia31, and the concentration applied proved safe when repetitively applied in monthly intervals32. Given the relatively high neurotoxicity of Mn2+ 9, future studies are required to define if this strategy is sensitive enough to detect ON pathologies already in early states when applied in tolerable concentrations. Such research will be useful to support clinically relevant MEMRI applications, e.g., for the diagnosis of multiple sclerosis and other neuropathies.
In summary, our study demonstrates that MEMRI is a powerful experimental approach to study retino-tectal circuitries in mice, thus extending optometric tasks for assessing the functionality of the visual system.
The authors have nothing to disclose.
A.K. is supported by the Oppenheim Foundation and R.H. is supported by the Velux Foundation. We thank I. Krumbein for technical and K. Buder for histological support, and J. Goldschmidt (Leibniz Institute for Neurobiology, Magdeburg, Germany) for technical advice on TIMM staining.
Manganese (II) chloride solution 1M | Sigma Aldrich, Taufkirchen, Germany | M1787 | MEMRI contrast reagent |
Conjuncain | Dr. Mann Pharma, Berlin, Germany | PZN 7617666 | 0.4% oxybuprocaine hydrochloride |
Floxal eye drops | Dr. Mann Pharma, Berlin, Germany | PZN 3820927 | 3 mg/ml ofloxacin |
Ointment panthenol | Jenapharm, Jena, Germany | PZN 3524531 | |
Chloral hydrate | Sigma Aldrich, Taufkirchen, Germany | C8383 | 420-450 mg/kg body weight |
Isoflurane | Actavis, Munich, Germany | PZN 7253744 | |
Hamilton syringe | Hamilton Company, Reno, NV, USA | 7634-01 | SYR 5 µl, 75 RN, no NDL |
34 G needle (34/35/pst4/tapN) | Hamilton Company, Reno, NV, USA | 207434/00 | removable needle RN, 34 gauge, lenght 38.1 mm, point style 4 |
Binocular Stemi-2000 | Zeiss, Oberkochen, Germany | ||
3T MRI scanner Magnetom TIM Trio | Siemens Medical Solutions, Erlangen, Germany | ||
Rat head coil | Doty Scientific Inc., Columbia, SC, USA | ||
Mouse holder | custom made | ||
Red light lamp | |||
Frozen section medium NEG-50 | Thermo Fisher Scientific, Schwerte, Germany | 6502 | tissue embedding for cryo-sections |
Sodium dihydrogen phosphate monohydrate (NaH2PO4) | Merck, Darmstadt, Germany | 106346 | for sulfide perfusion |
Sodium sulfide nonahydrate (Na2S × 9 H2O) | Sigma Aldrich, Taufkirchen, Germany | 208043 | |
gum arabic | Roth, Arlesheim, Switzerland | 4159 | for TIMM staining |
Hydroquinone (C6H6O2) | Roth, Arlesheim, Switzerland | 3586 | |
Citric acid (C6H8O7) | Roth, Arlesheim, Switzerland | 6490 | |
Tri-sodium citrate dihydrate (C6H5Na3O7 x 2H2O) | Merck, Darmstadt, Germany | 106448 | |
Silver nitrate (AgNO3) | Roth, Arlesheim, Switzerland | 7908 |