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The Journal of Neuroscience, March 1, 2003, 23(5):1949
Serum Transthyretin Monomer as a Possible Marker of Blood-to-CSF Barrier Disruption
Nicola Marchi1, Vince Fazio1, Luca Cucullo1, Kelly Kight1, Thomas Masaryk2, 3, Gene Barnett3, 5, Michael Volgelbaum3, 5, Michael Kinter4, Peter Rasmussen3, Marc R. Mayberg1, 3, 5, and Damir Janigro1, 3, 4, 5 1 Division of Cerebrovascular Research, Departments of 2 Radiology, 3 Neurosurgery, 4 Cell Biology and 5 Brain Tumor Institute, Cleveland Clinic Foundation, Cleveland, Ohio 44196
ABSTRACT
TOP
ABSTRACT
Introduction
The CNS is shielded from systemic influences by two separate barriers, the blood-brain barrier (BBB) and the blood-to-CSF barrier. Failure of either barrier bears profound significance in the etiology and diagnosis of several neurological diseases. Furthermore, selective opening of BBB tight junctions provides an opportunity for delivery of otherwise BBB impermeant drugs. Peripheral assessment of BBB opening can be achieved by detection in blood of brain-specific proteins that extravasate when these endothelial junctions are breached. We developed a proteomic approach to discover clusters of CNS-specific proteins with extravasation into serum that correlates with BBB openings. Protein profiles from blood samples obtained from patients undergoing iatrogenic BBB disruption (BBBD) with intra-arterial hyperosmotic mannitol were compared with pre-BBB opening serum. A low molecular weight protein (14 kDa) identified by mass spectroscopy as transthyretin (TTR) consistently correlated with BBBD. Protein gel electrophoresis and immunodetection confirmed that TTR was indeed extravasated in its monomeric form when CNS barriers were breached. The time course of TTR extravasation was compared with release from the brain of another BBB integrity marker, S-100
(11 kDa). Kinetic analysis revealed that the appearance of S-100
Key words: MRI; neurological disorders; choroid plexus; cerebral blood flow; neurodegeneration; neuroinflammation
Introduction
Loss of blood-brain barrier (BBB) function is an etiologic component of many neurological diseases. An intact BBB may restrict the delivery of certain therapeutic substances to the brain. Thus, measuring BBB function may be important to diagnose disease progression and monitor time-dependent changes in BBB integrity when chemotherapic penetration may be enhanced. At present, only invasive and expensive techniques such as contrast-enhanced magnetic resonance imaging, computed tomography (CT) scan, and lumbar puncture are available to clinically assess BBB integrity. An alternative approach has been proposed, consisting of detection of changes in blood composition that indicate BBB disruption (Kapural et al., 2002
).
Current BBB assessment by imaging or CSF sampling is based on direct or indirect determination of protein permeability across the BBB. CNS proteins are normally asymmetrically distributed, with generally much high concentration in plasma than in CSF. Thus, the appearance of plasma proteins in CSF is a hallmark of numerous CNS disorders with presumed or overt BBB disruption. Only a few proteins are synthesized exclusively by, or are present in, higher concentrations in CSF or interstitial compartment compared with the blood. These CSF markers may appear or increase their plasma concentration after passage across a failed BBB. Therefore, measuring levels of CSF proteins in plasma may be a reliable way to monitor blood to CNS barrier integrity without the use of invasive methods.
S-100
Materials and Methods
BBB disruption. The Cleveland Clinic Brain Tumor Institute provides a treatment called blood-brain barrier disruption (Neuwelt et al., 1991
Protein analysis. Sucrose gradient separation was performed to divide proteins by molecular weight. Ten milliliters of discontinuous 10/25/40% gradient and 200 µl of sample (75 µl of serum, 125 µl of gradient buffer) were used. The upper fraction was collected after 16 hr of centrifugation at 4°C (225,0000 × g). The low molecular weight fraction was filtered with a 3 kDa molecular weight cutoff (Amicon Centricon YM 3000) for 6 hr (5800 × g) to remove sucrose. Both SDS and NO-SDS-PAGE were used. Non-SDS-PAGE samples were analyzed in non-denaturing conditions.
Identification of TTR protein was performed by Western blotting techniques. Serum samples obtained from the BBBD procedures and protein were probed overnight at 4°C with primary TTR rabbit anti-human antibody (1:1000; Dako). Protein concentration was estimated according to the Bradford assay method. Relative expressions of proteins were determined by densitometric analysis using Scion Image Software. This approach was used to quantify the TTR and haptoglobin data shown in Figure 3. Radial immunodiffusion (RID) was used to quantitatively determine TTR in serum. Prefabricated immunodiffusion plates were purchased from Kent Laboratories (Bellingham, WA). Experiments were performed as recommended by the vendor.
For mass spectroscopy we used a liquid chromatography-mass spectroscopy (LC-MS) system Finnigan LCQ-Deca ion trap mass spectrometer system with a Protana microelectrospray ion source interfaced to a self-packed 10 cm × 75 µm inner diameter Phenomenex Jupiter C18 reversed-phase capillary chromatography column. Data were analyzed by using all collision-induced dissociation spectra collected in the experiment to search the National Center for Biotechnology Information nonredundant database with the search program TurboSequest. All matching spectra were verified by manual interpretation. The interpretation process was also aided by additional searches using the programs Mascot and Fasta, performed as needed.
Statistical methods. Data are presented as means ± SEM. ANOVA was need to determine significance. Origin 7.0 (Microcal) was used for statistical analysis.
Results
We tested blood samples from three patients affected by primary brain lymphoma who underwent monthly hemispheric BBBD by intra-arterial infusion of 1.4 M mannitol before receiving intra-arterial methotrexate (Neuwelt et al., 1980
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Figure 1. Schematic representation of the experiments described herein. A, Schematic representation and anatomic correlates of intra-arterial injection of hyperosmotic media and chemotherapeutic agents used to treat primary brain lymphomas with blood-brain barrier disruption. Hemispheric opening of the BBB was achieved after this procedure. B, The success of the procedure was quantified by CT scans taken approximately after completing the injection protocol. Note the hemisphere enhancement by iodinated contrast media indicated by arrows.
2-D gel electrophoresis
Two-dimensional electrophoresis is a powerful technique for separating proteins by iso-electric point and molecular weight (Molloy, 2000
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Figure 2. Detection of putative BBB markers by 2D gel electrophoresis of human blood proteins before and after osmotic opening of the BBB by intra-arterial mannitol. The samples used for loading were taken before mannitol injection and after chemotherapy. The timing of the injection of the osmotic agent and the introduction of the chemotherapic agent (methotrexate) are shown in the timeline. Protein signals that remained unchanged are indicated by arrows. The region in which significant changes were observed is boxed by a dashed line. Note the appearance of a distinct spot after BBB disruption. This spot corresponded to a protein of approximate molecular weight of 14 kDa and a pI of 5.5.
Comparison of gels prepared with pre-BBBD and post-BBBD was achieved by use of automated computer software. A number of strategies were used to ensure that the changes in protein levels were caused by BBB opening and not random fluctuations. First, we considered significant only the appearance of detectable spots ex novo and excluded increased levels of preexisting proteins. This criterion was used to minimize the possibility of uneven loading of gels as cause for the observed changes. Second, we excluded from further analysis changes that were not consistently observed in all BBBD. Thus, only spots that consistently appeared in post-BBBD gels in all three patients were further analyzed. Finally, we were limited to the identification of proteins that were amenable for mass spectroscopy analysis on Coomassie-stained gels.
A 14 kDa and 5.5 pI protein appeared after all BBBD procedures (Fig. 2). The size of the Coomassie-stained spot was quantified by proteomic software (Fig. 3). The asterisks indicate the actual time points at which the samples used for the gels were taken. This protein was subsequently identified as TTR (see below). Previous results demonstrated that opening of the BBB by osmotic means causes a reproducible increase in serum levels of S-100
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Figure 3. Time course of serum protein changes after BBB disruption. S-100
Molecular nature of the putative marker
After obtaining quantitative results describing protein changes, we investigated the qualitative nature of the low molecular weight protein shown in Figure 2. Protein identification was performed by LC-MS microelectroscopy mass spectroscopy. The region of interest was cut out from the gel and digested overnight with trypsin. The digest was analyzed by mass spectroscopy to determine peptide molecular weight and amino acid sequence. An additional spot (haptoglobin) was also processed to standardize the procedure for each individual gel. The polypeptide fragments obtained after digestion are shown in Table 1.
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Table 1. Maldi-mass Spectroscopy All of the fragments matched perfectly with the sequence of human transthyretin, formerly known as pre-albumin (NBCI 4507225). In addition, the molecular weight and isoelectric point of the spot identified in Figure 2 corresponded to the monomeric form of TTR. Transthyretin is the major protein product of the choroid plexuses and represents 20% of the total amount of protein in CSF (Hamilton and Benson, 2001
Immunological characterization of serum transthyretin
To confirm that the protein spot identified by the BBBD procedure was indeed human transthyretin, we performed Western blot analysis on samples taken from the same patients used for 2-D gel electrophoresis (Fig. 4). Samples processed under denaturing conditions displayed increased TTR immunoreactivity consistent with increased monomeric and dimeric TTR levels after BBBD. A commercially available TTR tetramer (55 kDa) was used as reference and loaded in the gel after processing under identical conditions. After denaturation, both dimeric and monomeric bands were identified by comparison with molecular weight standards. Furthermore, we used an alternative immunodetection approach based on quantitative RID of the sample in a gel containing antibody TTR. This test was performed, in contrast, on nondenaturated protein; however, the observed increase in TTR as detected by RID does not necessary imply that the monomeric form of TTR was indeed increased in plasma.
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Figure 4. Immunological analysis of protein changes induced by BBB disruption. Top panel, Denaturated proteins were run in parallel with purified TTR (left lane). Western blot analysis revealed a significant increase of immunosignal for both low molecular weight isoforms. Quantitative analysis was performed on the same samples by RID (bottom panels); note the progressive increase of the immunoprecipitation signal surrounding the sample port (see Materials and Methods for details). The numeric values represent TTR levels extrapolated from these measurements and are expressed as micrograms per milliliter.
Because the tests described above were performed either under conditions that do not allow preservation of native protein structure (e.g., monomer vs tetramer) or by RID, we performed additional experiments on nondenatured proteins obtained from identical samples and separated by their molecular weight (Fig. 5). Purified TTR was again loaded as reference. Note that even under nondenatured conditions, a sharp increase in a band consistent with the monomeric form of TTR occurred after BBB disruption. Also note that this band was virtually absent before the BBBD, confirming that the monomeric form of TTR is present predominately in the CSF.
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Figure 5. Non-SDS separation of pre-BBBD and post-BBBD samples. Low molecular weight proteins obtained after separation with a sucrose gradient (cutoff 50 kDa) were loaded on a non-denaturating gel. Note the appearance of a 15 kDa molecular weight band after BBB disruption. Also note that this band corresponds to the monomeric form of standard TTR loaded on a separate gel.
Discussion
The main aim of the experiments described herein was to develop a technique that allows detection of novel serum markers indicative of breaching of the cellular barriers that normally shield the brain from systemic influences. We discovered a new marker of barrier integrity, transthyretin, by combing proteomic strategies with clinical procedures during which the BBB is disrupted to allow penetration of chemotherapic agents to treat brain tumors. Both mass spectroscopy and immunoblotting confirmed that TTR is increased early (minutes) after BBB disruption. However, the time course of TTR extravasation from CSF to plasma lagged behind that of another BBB marker, S-100
Proteomics and BBB markers
The original discovery of the usefulness of S-100
Plasma electrophoresis has been used to diagnose human diseases. Conversely, CSF protein analysis has been instrumental in understanding CNS disorders (Reiber, 2001
Significance of CNS barriers
The barrier that separates the blood from the cerebral interstitial fluid is defined as the BBB, whereas the barrier that separates the blood and CSF (BCSFB) discontinues the circulation between the blood and CSF (Davson and Segal, 1995
Recent evidence suggests that the opposite phenomenon, i.e., leakage of CSF-specific proteins into blood, may also be used to detect BBB integrity (Kapural et al., 2002
Transthyretin and CNS barriers
Transthyretin represents a disproportionate fraction (25%) of CSF protein, prompting the suggestion that it is either selectively transported across the blood-CSF barrier or synthesized de novo within the CNS (Schussler, 2000
In the blood, TTR is usually present in its tetrameric form and originates from liver secretion (Hamilton and Benson, 2001
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Figure 6. Different distribution between S-100
Although the appearance of S-100
There are several issues that need to be addressed concerning the putative role of TTRmonomer as a peripheral marker of BCSF barrier integrity. For example, opening of the CNS barriers with mannitol for chemotherapic purposes was followed by injection of the anti-neoplastic agent methotrexate. It is thus possible that methotrexate may be involved in the release process of TTR from the CNS compartment to plasma. This seems highly unlikely on the basis of experiments in which samples were taken from patients undergoing intra-arterial chemotherapy without mannitol-induced BBB disruption. In these samples, no detectable changes in S-100
To directly follow the process of extravasation of tracer molecules from the blood to the brain and vice versa, one should ideally compare changes occurring simultaneously in plasma and CSF (Stanness et al., 1996
In conclusion, we have shown that the TTRmonomer is a candidate marker for blood-to-CSF barrier dysfunction, in a manner similar to S-100
FOOTNOTES Received Sept. 23, 2002; revised Nov. 26, 2002; accepted Dec. 13, 2002.
This work was supported in part by the National Institutes of Health (NIH-NS43284, NIH-HL51614, and NIH-NS38195). We also thank Dr. Anne-Charlotte Aronsson for continuous support and encouragement, and Luca Cucullo, Matteo Marroni, and Barbara Aumayr for helpful discussion. Sangtec Medical (Bromma, Sweden) provided the kits for immunodetection of NSE and S-100
Correspondence should be addressed to Dr. Damir Janigro, Cerebrovascular Research, NB-20 Lerner Research Institute, Cleveland Clinic Foundation, 9600 Euclid Avenue, Cleveland, OH 44196. E-mail: janigrd{at}ccf.org.
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