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Previous Article | Next Article
The Journal of Neuroscience, January 15, 2002, 22(2):536-545
Anterograde Transport of Tumor Necrosis Factor-
in the Intact and Injured Rat Sciatic Nerve
Maria Schäfers1, 2, Christian Geis1, Dominik Brors3, Tony L. Yaksh2, and Claudia Sommer1 1 Department of Neurology, University of Würzburg, 97080 Würzburg, Germany, and 2 Anesthesiology Research Laboratory and 3 Department of Otolaryngology and Neuroscience, University of California San Diego, La Jolla, CA 92093
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Tumor necrosis factor-
(TNF) appears as a key player at both central and peripheral terminals in early degenerative pathology and pain behavior after peripheral nerve injury. Recent studies suggest that TNF may be axonally transported and thereby contribute to these central and peripheral actions. To characterize this transport, we used a double ligation (DL) procedure that distinguishes between anterograde and retrograde flow to visualize the axonal transport of endogenous TNF compared with the neurotrophin nerve growth factor (NGF) and to the neuropeptide calcitonin gene-related peptide (CGRP). In the intact nerve, TNF and CGRP immunoreactivity predominantly accumulated proximal to the DL (anterograde transport), whereas NGF displayed exclusive retrograde transport. At 20 hr after chronic constrictive injury (CCI), the anterograde transport of TNF and CGRP to the nerve injury site was dramatically increased. The results were corroborated by the analysis of axonal transport of exogenously applied 125I-TNF and 125I-NGF. After intraneural injection, 125I-TNF accumulated proximally to a DL, suggesting anterograde transport. In the unligated nerve, 125I-TNF was specifically transported anterogradely to the innervated muscle but not to skin. After CCI, 125I-TNF accumulated proximally to the peripheral nerve injury site, and endogenous TNF was exclusively increased in medium-sized and large dorsal root ganglion (DRG) neurons, suggesting that DRG neurons are a major contributing source of increased TNF traffic in the injured sciatic nerve. Our results suggest that anterograde transport of TNF plays a major role in the early neuronal response to peripheral nerve injury at sites distal to the cell body.
Key words: TNF; axonal transport; chronic constrictive injury; NGF; CGRP; dorsal root ganglion
INTRODUCTION
Pharmacological and physiological studies suggest that proinflammatory cytokines such as tumor necrosis factor-
,b
In this study, we examined the axonal transport of endogenous and exogenously applied TNF in the intact and chronically constricted rat sciatic nerve. In the intact nerve, we found an exclusive and rapid anterograde transport of TNF to the muscle but not to skin. After chronic constrictive injury (CCI), the anterograde transport of TNF was strongly increased and stopped at the peripheral nerve injury site. Endogenous TNF was expressed in predominantly small DRG neurons in the intact nervous system, whereas after CCI exclusively medium-sized and large DRG neurons upregulated their expression of TNF. It seems likely that DRG sensory neurons are one of the major contributing sources for increased TNF anterograde transport after nerve injury.
MATERIALS AND METHODS
Animals. Female Sprague Dawley rats (200-250 gm, in total n = 128) were obtained from Charles River (Sulzfeld, Germany). The animals were housed on a 14 hr/10 hr light/dark cycle with standard rodent chow and water ad libitum. Experimental groups were composed as follows: (1) experiments of endogenous axonal transport of TNF, nerve growth factor (NGF), and calcitonin gene-related peptide (CGRP) (n = 15); (2) experiments of exogenous axonal transport with 125I-TNF (n = 84) and 125I-NGF (n = 11); and (3) experiments of double immunofluorescence in the DRG (n = 6) and sciatic nerve (n = 12). The several experimental paradigms are described in Figure 1.
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Figure 1. Schematic of the experimental treatments used to determine the axonal transport of endogenous (A, B) and exogenously applied 125I-labeled (C-G) TNF. To visualize anterograde and retrograde transport of endogenous TNF, NGF, and CGRP, we performed a DL procedure (A, B). To analyze the axonal transport before and after experimental mononeuropathy, some rats received additionally a bilateral CCI made 1 d earlier (B, E). For the study of exogenously applied 125I-TNF and 125I-NGF, the following paradigms were used: C, the radioligands were injected into a double-ligated rat sciatic nerve; D, the radioligands were injected into the intact sciatic nerve; E, the radioligands were injected 2 mm proximally to a CCI of the sciatic nerve made 1 d earlier; and F, G, the radioligands were injected into the gastrocnemius muscle (F) or plantar skin (G). As illustrated by the dotted boxes, the ipsilateral and contralateral sciatic nerve, gastrocnemius muscle, plantar skin, lumbar DRG, and spinal cord were dissected for detection of radioactivity after 6 and 20 hr or 3 d. In the sciatic nerve, 2 mm segments were separately analyzed.
Surgery. All surgical procedures used herein were performed under deep barbiturate anesthesia using sodium pentobarbital given intraperitoneally at a dose of 50 mg/kg. To visualize anterograde and retrograde transport of endogenous TNF, NGF, and CGRP, we performed a double ligation (DL) procedure that has been used previously to examine the axonal transport of acetylcholinesterase, neurotransmitters, and neurotrophins in the sciatic nerve (Ranish and Ochs, 1972
To analyze the axonal transport before and after experimental mononeuropathy, some rats received a bilateral CCI as described previously (Sommer and Schäfers, 1998
Axonal transport of endogenous TNF, CGRP, and NGF. After 20 hr or 2 d, the double-ligated nerve was removed for immunostaining. For studies of axonal transport of endogenous TNF, NGF, and CGRP, sciatic nerve tissue was harvested in untreated rats and in rats whose sciatic nerve was constricted 1 d earlier. Frozen longitudinal cryostat sections at the level of the ligation were cut at 10 µm, mounted on slides, and incubated overnight at 4°C with a polyclonal rabbit anti-rat TNF antibody (Serotec, Oxford, UK), a rabbit anti-rat NGF antibody (Chemicon, Hofheim, Germany), or a rabbit anti-rat CGRP antibody (Peninsula, Heidelberg, Germany). An ABC system (Vector Laboratories, Burlingame, CA) and 3,3' diaminobenzidine tetrahydrochloride were used for detection. Controls included omission of primary antibody (AB) and, in the case of TNF, preabsorption with the antigen.
Axonal transport of exogenous 125I-TNF and 125I-NGF. For studies of axonal transport of exogenously applied TNF, rat 125I-TNF (Amersham Biosciences, Freiburg, Germany; specific activity, 400-1200 Ci/mmol) was used to evaluate and quantify the uptake and transport of TNF from within the sciatic nerve, gastrocnemius muscle, or plantar skin. All injections were performed under barbiturate anesthesia. In one group of rats, 125I-TNF was injected into the rat sciatic nerve, which was either double-ligated or untreated (Fig. 1C,D, respectively). In another group, the sciatic nerve was chronically constricted 1 d before injection, and 125I-TNF was injected 2 mm proximally to the CCI (Fig. 1E; in all intraneural injections, 3 µCi, in a volume of 5 µl). In another group, 125I-TNF was injected into gastrocnemius muscle or plantar skin (Fig. 1F,G, respectively; for both treatments, 1.5 µCi in a volume of 50 µl). 125I-NGF was used as a positive control for exclusive retrograde axonal transport within the sciatic nerve. Six or 20 hr or 3 d after injection of the radioligands, ipsilateral and contralateral sciatic nerve tissue (Fig. 1C-G), gastrocnemius muscle (Fig. 1D,E), plantar skin (Fig. 1D,E), and L4 and L5 DRG and lumbar spinal cord (Fig. 1D-G) were dissected. To follow the movement of the radioligands, each sciatic nerve was cut into 10 equal nerve segments (each 2 mm). To assess systemic distribution of radioactivity by blood flow, samples of liver, lung, and blood gained by intracardial extraction were dissected from rats of each of the different treatment groups. Radioactivity was measured in all samples directly. Each sample was counted for 5 min in a gamma counter, and background was subtracted.
Endogenous TNF in the rat sciatic nerve and DRG before and after CCI. Sciatic nerve tissue was harvested from uninjured rats and rats 3 and 12 d after CCI. Three-millimeter-long sciatic nerve segments distal to the ligatures and corresponding segments from the controls were deep-frozen and processed for histology. Immunofluorescence was performed on 12 µm cryosections with a polyclonal rabbit anti-mouse TNF AB (Serotec; 1:500). For double immunofluorescence with TNF, a monoclonal mouse anti-rat S100 AB (Chemicon; 1:100) or monoclonal mouse anti-rat ED-1 AB (Serotec; 1:2000) was used as primary AB. A Cy3-conjugated secondary AB (Amersham; 1:500) and Cy2-labeled secondary AB (Amersham; 1:500) were used for detection. Lumbar DRGs (L4 and L5) were harvested in uninjured rats and in rats 4 d after CCI. Every 10th section of serial 10 µm cryosections of the L5 ganglion was immunostained for TNF with a Cy3-conjugated secondary AB (Amersham; 1:500) and isolectin IB4 (Sigma, St. Louis, MO; 1:50) with an ExtrAvidin-conjugated secondary AB (Sigma; 1:100). This resulted in an average of 15 stained sections per ganglion.
Morphometry. The immunostained DRG sections were viewed and digitized at a magnification of 100× with a Zeiss (Oberkochen, Germany) Axiophot 2 microscope using a fully motorized scanning table (Märzhauser) and Image Pro Plus (version 4.0) software (Media Cybernetics Inc., Silver Spring, MD). A density threshold was set to identify the immunoreactive neuronal profiles. The number and cross-sectional area of the immunoreactive profiles were measured and expressed in a histogram.
Statistical analysis. Comparisons of the amount of radioactivity of different tissues and morphometric data were performed by using repeated measures ANOVA followed by a least significant difference post hoc test (Stat View 5.0). References associated with p < 0.05 were considered statistically significant. All data are given as mean ± SE.
RESULTS
Increased anterograde transport of endogenous TNF after chronic constriction injury
To examine the transport of endogenous TNF in the retrograde or anterograde direction, we used the DL technique. To validate this approach, we examined NGF and CGRP accumulation by immunohistochemistry. At 20 hr after placement of the DL, NGF-IR was visible on the distal side of the distal ligature (Fig. 2B) and on the distal side of the proximal ligature (Fig. 2A), confirming its exclusive retrograde axonal transport (Palmatier et al., 1984
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Figure 2. Immunohistochemical staining of endogenous NGF in the rat sciatic nerve proximal (PROX) and distal (DIST) to a DL 20 hr after placement. The proximal (central) side is on the left, and the distal (peripheral) side is on the right. A, B, In the double-ligated but otherwise intact nerve, endogenous NGF is accumulating distally to the DL, suggesting exclusive retrograde transport (arrows). C, D, After chronic constriction injury made 1 d earlier distally to the DL, the distal accumulation of NGF immunoreactivity is moderately increased (arrows). Scale bar, 100 µm.
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Figure 3. Immunohistochemical staining of endogenous CGRP in the rat sciatic nerve proximal (PROX) and distal (DIST) to a DL 20 hr after placement. As in Figure 2, the proximal (central) side is on the left, and the distal (peripheral) side is on the right. A, B, Endogenous CGRP is accumulating proximally and distally to the DL 20 hr after placement of the ligatures (arrows). C, D, After chronic constrictive injury, the accumulation proximally to the proximal ligature is markedly increased (C, arrow) without a significant change distally to the ligature (D), suggesting increased anterograde transport. Scale bar, 100 µm.
TNF-IR accumulated distally and proximally to both ligatures 20 hr after placement (Fig. 4A,B), suggesting retrograde and anterograde axonal transport in the double-ligated but otherwise intact sciatic nerve. CCI resulted in a significant increase of TNF-IR proximal to the proximal ligation (Fig. 4C), suggesting upregulated anterograde transport of endogenous TNF after CCI. Distal to the distal ligature or between both ligatures, there was no additional increase of the TNF-IR after CCI, indicating no increase of retrograde transport (Fig. 4D).
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Figure 4. Immunohistochemical staining of endogenous TNF in the rat sciatic nerve proximal (PROX) and distal (DIST) to a DL 20 hr after placement. As in Figures 2 and 3, the proximal (central) side is on the left, and the distal (peripheral) side is on the right. A, B, Endogenous TNF is accumulating proximally and distally to the DL after placement of the ligatures (arrows). C, D, After chronic constriction injury, the proximal accumulation of endogenous TNF is markedly increased (arrow), whereas the distal accumulation of TNF remains unchanged. Scale bar, 100 µm.
Anterograde transport of exogenous 125I-TNF in the intact nerve: accumulation of anterogradely transported 125I-TNF proximally to the nerve injury
The immunohistochemical results were corroborated by the analysis of the axonal transport of exogenously applied 125I-TNF and 125I-NGF. To validate this approach, 125I-NGF was injected into the double-ligated sciatic nerve (Fig. 1C), and radioactivity was detected 20 hr later (Fig. 5A). 125I-NGF radioactivity was three times greater in the nerve segment distal to the proximal ligature (L1, segment
4) than in the segment proximal to the distal ligature (L2, segment +4; p < 0.05) and five times greater than in the nerve segment proximal to the proximal ligature (L1, segment
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Figure 5. Distribution of 125I in 2 mm segments of the rat sciatic nerve 20 hr after intraneural injection (INJ) of 125I-NGF (A) or 125I-TNF (B) between a double ligature. The double ligature was placed before injection; the proximal (central) ligature (L1) is on the left, and the distal (peripheral) ligature (L2) is on the right. Data represent mean counts per minute (CPM) ± SEM for each nerve segment. A, After injection of 125I-NGF, 125I accumulates distally to the proximal ligature (L1) but not proximally to the distal ligature (L2), suggesting exclusive retrograde transport (*p < 0.05 for segment
After injection of 125I-TNF into an intact sciatic nerve (Fig. 6A), radioactivity accumulated significantly in the sciatic nerve segments distally to the injection (segments +4, +6, and +8 vs segments
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Figure 6. Distribution of 125I in 2 mm segments of the rat sciatic nerve after intraneural injection of 125I-TNF in an intact rat sciatic nerve (A) or 2 mm proximal to a CCI (B; gray bars) made 1 d earlier. The proximal (central) side is on the left, and the distal (peripheral) side is on the right. A, In the intact nerve, the nerve segments peripheral to the injection site significantly accumulate 125I, suggesting anterograde transport. This accumulation is maximal after 6 hr (*p < 0.05 for segments 4, 6, and 8 vs segments
No retrograde transport of 125I-TNF after intramuscular, intradermal, or intraneural injection
To examine whether skin or muscle afferents were involved in the axonal transport of 125I-TNF, rats were injected intradermally in the foot or into the gastrocnemius muscle with the sciatic nerve intact (Fig. 1F,G). When 125I-NGF was used as a positive control for retrograde transport, radioactivity significantly accumulated in all ipsilateral sciatic nerve segments and DRG 20 hr after intramuscular and intradermal injection (data not shown). After intramuscular or intradermal injection of 125I-TNF, there was no accumulation of radioactivity in the sciatic nerve segments or in the DRG or spinal cord 6 and 20 hr and 3 d after injection, suggesting no retrograde transport of 125I-TNF in skin or muscle afferents to the sciatic nerve (data not shown).
To examine whether endoneurial 125I-TNF was transported retrogradely to the DRG or spinal cord, 125I-TNF was injected into the intact rat sciatic nerve. When 125I-NGF was used as a positive control for retrograde transport, radioactivity significantly accumulated in the ipsilateral DRG. This accumulation was blocked by DL placed on the nerve immediately before intraneural injection (Fig. 7A; p < 0.05 ipsilateral DRG in the intact nerve vs ipsilateral DRG with DL). After intraneural injection of 125I-TNF, there was no accumulation of 125I in the ipsilateral DRG or spinal cord (Fig. 7B).
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Figure 7. Distribution of 125I in the lumbar DRG and spinal cord (SC) 20 hr after intraneural (i.n.) injection of 125I-NGF or 125I-TNF into the rat sciatic nerve. A, After injection of 125I-NGF, 125I significantly accumulated in the ipsilateral DRG but not in SC, suggesting retrograde transport to the DRG. This transport could be inhibited by placement of a DL around the injection site (*p < 0.05 for ipsilateral DRG after injection into the intact vs double-ligated nerve). B, After injection of 125I-TNF in the intact, double-ligated, or chronically constricted nerve, there was no accumulation of 125I in the DRG or SC. CPM, Counts per minute.
Early anterograde transport of exogenous 125I-TNF to the innervated muscle
Potential targets of anterogradely transported TNF are the innervated skin or muscle. To consider these potential targets, 125I-TNF was injected into the intact sciatic nerve, and radioactivity was measured in plantar skin and gastrocnemius muscle. Six and 20 hr after intraneural injection of 125I-TNF, 125I accumulated in the ipsilateral gastrocnemius muscle, with an early maximum after 6 hr (p < 0.001 for ipsilateral vs contralateral after 6 hr; Fig. 8A). To examine the influence of nerve injury on anterograde transport of TNF to the muscle, 125I was analyzed 20 hr after intraneural injection of 125I-TNF 2 mm proximally to a CCI or DL made 1 d earlier (Fig. 8B). Both types of ligature reduced accumulation of 125I in the ipsilateral muscle significantly (p < 0.05 for ipsilateral muscle with intact nerve vs ipsilateral muscle after DL and ipsilateral muscle after CCI). Unlike the muscle, there was no accumulation of 125I in the ipsilateral skin with an intact or injured sciatic nerve (Fig. 8C).
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Figure 8. Distribution of 125I in the gastrocnemius muscle or plantar skin after intraneural (i.n.) injection of 125I-TNF. A, Temporal course of accumulation of 125I in the ipsilateral and contralateral gastrocnemius muscle. After 6 hr, the ipsilateral gastrocnemius muscle shows a significant increase of 125I-TNF (***p < 0.001 for ipsilateral vs contralateral gastrocnemius muscle), suggesting fast anterograde transport. After 20 hr there is still a trend of accumulation in the ipsilateral gastrocnemius muscle, which is not statistically significant. B, The accumulation of 125I in the ipsilateral gastrocnemius muscle 20 hr after injection can be blocked by a DL or CCI of the sciatic nerve made before the injection, suggesting axonal transport (*p < 0.05 for intraneural injection in the intact nerve vs intraneural injection within a DL or proximally to a CCI). C, There is no accumulation of 125I in the plantar skin after injection of 125I-TNF into the intact, double-ligated, or CCI-lesioned sciatic nerve. CPM, Counts per minute.
Potential sources of anterogradely transported TNF
Potential sources of anterogradely transported TNF are DRG sensory neurons, motor neurons, or Schwann cells within the nerve. Some evidence suggests expression of TNF in motor horn cells (DeLeo et al., 1997
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Figure 9. Double immunofluorescence for endogenous TNF in the rat sciatic nerve and lumbar DRG before and after CCI. A, B, Twelve micrometer cryosections of rat sciatic nerve immunostained for TNF and S-100 (Schwann cell antigen). TNF-immunoreactive structures appear red; S-100-immunoreactive structures appear green; and colocalization of the antigens appears orange. A, In the uninjured nerve, TNF-IR is shown in Schwann cells of myelinated (arrows) and unmyelinated (arrowheads) axons. B, In a 12 µm sciatic nerve 3 d after CCI, the number of TNF-IR Schwann cells has greatly increased (arrows, arrowheads). C, D, Ten micrometer cryosection of rat DRG 4 d after CCI, immunostained for TNF (red) and isolectin IB4 (green). Small DRG neurons are immunoreactive for TNF; some of them are also IB4 positive (asterisks). Other small DRG neurons are IB4-positive but not TNF-positive (arrows). In addition, medium-sized and large DRG neurons express TNF and are not IB4-positive (arrowheads).
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Figure 10. Histogram illustrating the size distribution of TNF-immunoreactive DRG neuronal profiles before (gray bars) and 4 d after (black bars) CCI. In the intact nervous system, most TNF-immunoreactive DRG cells are small. After CCI, TNF immunoreactivity is increased exclusively in medium-sized to large DRG neurons (*p < 0.05 for cells with a cross-sectional area between 600 and 1000 µm2, compared before and after CCI).
DISCUSSION
Anterograde transport of endogenous and exogenous TNF in the intact and injured peripheral nerve
We have presented several lines of evidence that TNF is anterogradely transported in the rat sciatic nerve. Using the double ligation approach, we demonstrated that endogenous TNF accumulated proximally to a ligation over 20 hr. This elevation did not reflect an overall increase in protein in the nerve, because there was no uniform distribution of TNF-IR in the nerve segment between the two ligations, indicating a lack of significant local TNF synthesis or influx. Exogenous intraneural injection of 125I-TNF into a double-ligated nerve resulted in significant accumulation proximal to the ligature. Injection of 125I-TNF into the intact nerve showed a significant increase of 125I-TNF in the distal but not proximal nerve segments. After intraneural injection of 125I-TNF, there was a time-dependent accumulation in the peripheral targets, which surprisingly was exclusively limited to the ipsilateral innervated muscle but not skin.
TNF anterograde transport of endogenous TNF was increased after nerve injury, concomitantly with increased TNF-IR in DRG neurons. Thus, one explanation for the increased amount of TNF transported to the proximal ligature may be the increased availability of the cytokine. Alternatively, as shown for neurotrophins (Tonra et al., 1998
Anterograde transport of CGRP was also increased after nerve injury in the present study. In a previous study with CCI, the axons spared by the injury increased the axonal transport of CGRP to the ipsilateral gracile nucleus (Ma et al., 1999
No evidence of retrograde transport of TNF to the DRG or spinal cord
In contrast to a recent study with exogenous biotinylated TNF (Shubayev and Myers, 2001
Fibers, targets, and possible sources of TNF anterograde transport
Axonal transport of TNF resulted in an early accumulation of 125I in the ipsilateral but not contralateral gastrocnemius muscle 6 hr after injection. The exclusive accumulation of 125I-TNF in the ipsilateral muscle but not in skin may suggest specific axonal transport of TNF in possibly medium-sized or even larger fibers. This is congruent with the fast transport rate of TNF, which is in accordance with the fast transport rate of most of the neurotrophins (Vallee and Bloom, 1991
There are several potential sources of anterogradely transported TNF. Within the peripheral nerve, non-neuronal cells, primarily Schwann cells, express TNF (Wagner and Myers, 1996a
Possible role of anterogradely transported TNF
There are several hypotheses for the physiological role played by anterogradely transported TNF. Because anterograde transport of endogenous TNF to the peripheral nerve injury site is increased after CCI, it may be relevant to pain-associated behavior after nerve injury. Anterogradely transported TNF accumulates in muscle but not in skin. Interestingly, axotomized and intact muscle afferents but not skin afferents develop ongoing activity of dorsal root origin after a peripheral nerve lesion (Michaelis et al., 2000
In conclusion, TNF is specifically transported to the innervated muscle, and after damage to the peripheral nerve, TNF anterograde transport is dramatically increased. The specificity of these findings suggests an important role for this cytokine in the function of the peripheral nervous system and in the response to nerve injury.
FOOTNOTES Received Aug. 20, 2001; revised Oct. 24, 2001; accepted Oct. 30, 2001.
This work was supported by Deutsche Forschungsgemeinschaft Grant SFB 353. We thank M. J. Lohse for the generous use of his radioactive facilities, C. Dees, L. Biko, and B. Dekant for expert technical assistance, and K. V. Toyka for helpful suggestions during the preparation of this manuscript.
Parts of this paper were presented at the 30th Annual Meeting of the Society for Neuroscience, New Orleans, LA, 2000.
Correspondence should be addressed to Dr. Maria Schäfers, Anesthesiology Research Laboratory, University of California San Diego, 9500 Gilman Drive, La Jolla, CA 92093. E-mail: mschaefers{at}ucsd.edu.
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