All publications and patent applications mentioned in this specification are herein incorporated by reference in their entirety to the same extent as if each individual publication or patent application was specifically and individually indicated to be incorporated by reference.
Atherosclerosis is an artery disease believed to arise from endothelial malfunction, accumulation of lipid materials in the intima of artery, inflammatory cell infiltration and reaction, artery wall structure damage, smooth muscle cell proliferation and fibrosis change. These factors may result in artery stenosis and ischemia of supplied organs and severe clinical consequences, such as heart attack in coronary artery stenosis, claudication and critical limb ischemia in occlusive peripheral vascular disease.
Atherosclerosis may be treated by atherectomy (e.g., removal of stenosed tissue). For example, directional atherectomy may use a catheter-based system to excise and retrieve plaque tissue for the transluminal treatment of coronary and peripheral atherosclerotic artery disease. The excision and collection of plaque tissue in directional atherectomy not only leaves behind a large and smooth lumen at the treated artery segment, but may also provide plaque tissue for histopathological analysis and new insights into the mechanism of atherosclerotic progress and variable therapy response.
Atherosclerotic stenoses in coronary and peripheral arteries vary widely in presentation and severity. In peripheral arteries the disease is under-diagnosed and under-treated, amputation rate in the US is staggering at 200,000 per year and recurrence rates following peripheral interventions (atherectomy, angioplasty and stenting) are still high. Peripheral stent fracture and failure of drug eluding stents in the periphery remains a big problem. The Baim-Kuntz coronary model of “bigger is better” has been difficult to apply to peripheral vessels because of the diffuse nature of the disease and the large atherosclerotic burden. A high capacity atherectomy system with on-board real-time imaging to guide plaque resection could potentially overcome the disadvantages in current devices and allow the Baim-Kuntz model to be applied to the peripheral vascular space for the first time.
As mentioned above it is well recognized that peripheral plaque burden is large in comparison to coronary lesions. Current atherectomy systems leave up to 60% of the atheroma atheroma in the vessel as confirmed by intra-vascular intra-sound (IVUS). A new image guided atherectomy (IGA) system with greater capacity for tissue management may be better able to safely achieve maximal luminal gain with minimal barotraumas. To achieve this improved acute outcome, a new cutter design combined with imaging near the cutter edge may be used. The method and devices described herein may help guide treatment with such a device, or even in devices that do not include cutting components and/or on-board imaging.
Despite high procedure success rates, excellent patency rate, and low complications, post-intervention restenosis often limits plaque excision methods from becoming a more routine and effective resvasculization procedure for the treatment of coronary and peripheral atherosclerotic artery disease. Thus, there is a need to understand the mechanism of restenosis, and to determine new approaches for preventing and treating post-intervention restenosis.
Although there have been other attempts to histopathologically analyze excised atherosclerotic plaque tissue, the results have generally proven unsatisfactory. For example, the relationship between plaque histopathological components and subsequent restenosis atherosclerotic lesions treated with directional atherectomy device has been controversial. Such plaque histopathological studies and evaluations have been mostly based only on the qualitative presence or absence of different plaque components. Quantitative histological analysis may provide more detail information to help understand the mechanism of restenosis. Herein we describe a method of describing and quantifying various atherosclerotic plaque elements, and devices for applying this analysis. Furthermore, we herein identify specific factors and parameters that correlate with angiographic restenosis rates in coronary atherosclerotic patients treated by directional atherectomy.
We have discovered that histopathological analysis of atherosclerotic artery tissue from patients with cardiovascular disease may be used to predict incidence of restenosis in the artery. More particularly, restenosis of may be predicted based on the histopathological analysis of atherosclerotic tissue (including excised fragments from atherectomy procedures) in patients with atherosclerotic artery disease. The histopathological analysis applied may be quantitative; furthermore, quantitative estimates and ranges are provided which may correlate to restenosis. Applications of the quantitative histological parameters and ranges of values of these parameters are also described.
The present invention relates to methods and devices for predicting restenosis, and for treating atherosclerosis to prevent or reduce the incidence of restenosis.
In particular, described herein are methods of predicting restenosis in a stenosed peripheral artery based on the quantitative histology of the vessel. For example, a method of treating a stenosed artery (and particularly a peripheral artery) may include the steps of determining a level of hypercellularity, and providing a predictive index of restenosis based on the level of hypercellularity and/or the level of lipid-rich tissue, and/or the level of inflammatory cells in the tissue. Each of these factors may be examined individually, or they may be combined.
These factors (e.g., hypercellularity, lipid-rich regions, inflammatory cells) may be provided as a quantitative and/or qualitative index. For example, hypercellularity may be provided as a percentage of total tissue or a percentage of hypercellularity, or the level of hypercellularity may be used to provide an indicator of “low/medium/high” or the like. An index indicating the likelihood of restenosis (either quantitatively or qualitatively) may be provided by combining one or more of these factors. These factors may also be combined with other factors, such as post-interventional minimal lumen diameter (MLD) to provide a more robust indicator of
Also described herein are systems and devices for treating or assisting in the treatment of stenosis by providing an indication of the hypercellularity, lipid-rich regions and/or inflammatory cells in an artery, and particularly a peripheral artery. Systems including visualization methods such as catheter-based imaging systems using Optical Coherence Tomography (OCT) are of particular interest. Systems may also be configured for predicting or indicating if restenosis is to occur. Systems or devices may be configured to show hypercellularity and/or lipid-rich tissue and/or inflammatory cells in an arterial tissue. The systems may be configured to present quantitative or qualitative estimates in real-time.
In some variations devices for treating atherosclerosis may be configured for eat-time or near real-time aging of tissue so that the artery may be treated while imaging the tissue. In general, these devices may be used with one more catheters for imaging and treating the tissue.
For example, described herein are devices for treating atherosclerosis and prevent restenosis. In some variations the devices include: an imaging catheter having a sensor configured to image a portion of an artery; a processor configured to receive images of the artery from the sensor processor and to detect regions of hypercellularity in the artery based on the received images, and further configured to detect regions of either or both: lipid-rich tissue and inflammatory cells in the artery from the received ages; and a display configured to display a modified view of the artery indicating hypercellularity and one or both of lipid-rich tissue and inflammatory cells in the artery.
The device imaging catheter, may be any appropriate catheter, including an atherectomy catheter. Steerable catheters, and catheters having more than one imaging modality may be included (or catheters having one imaging modality). For example, the imaging catheter may be an OCT imaging catheter and the sensor comprises an OCT imaging sensor.
The device (or systems) may include any appropriate processor or processors for taking and analyzing images of the arterial tissue or regions of the artery. A processor may be a dedicated or general purpose processor. The processor may be configured in part as a controller for controlling operation of the various components of the system. In some variations a separate controller may be used. The controller may control operation of the analysis and/or the display of images and the resulting identified tissue regions (e.g., showing regions at high risk for restenosis on a display). As mentioned, in some variations, the processor and display are configured to operate in real or near-real time.
The processor (or processors) may include logic for analyzing and/or controlling the system. For example a device or system may include detection logic configured to detect regions of hypercellularity and either or both: lipid-rich tissue and inflammatory cells in the artery from the received images. The detection logic may be further configured to estimate, measure or count a degree of hypercellularity and one or both of lipid-richness and/or the amount of inflammatory cells (e.g., macrophages, lymphocytes, etc.) in the tissue region. The device or system may also include index logic for calculating an index that combined (and/or weights) the measures, counts, or estimates of hypercellularity and one or both of lipid-richness and/or the amount of inflammatory cells (e.g., macrophages, lymphocytes, etc.) in the tissue region. In some variation the index logic may be included with the detection logic, or vice-versa.
The display may be a visual display, such as monitor, screen, projection, or the like. The display may be configured to highlight one or more regions of overlap indicating both hypercellularity and either or both: lipid-rich tissue and inflammatory cells in the artery on the modified view of the artery. In some variations the display may overlay an image of the artery or a region of the artery with an indication of the likelihood of restenosis, and my include markers indicating the relative location of the catheter or another device such as an atherectomy catheter or the cutting region of an atherectomy catheter. The indicator of the likelihood of restenosis may be a color (e.g., color intensity or color-coding) or numeric (0 to 100, 0 to 10, 0.00 to 1.00, etc.) or percentage indicator.
As mentioned, the processor further may also include index logic configured to determine an index of restenosis based on the degree of hypercellularity and either or both: the degree of lipid-rich tissue and the degree of inflammatory cells in the artery from a region of the artery in the received images. In some variations, the index logic determines the index of restenosis based on the degree of hypercellularity, the degree of lipid-rich tissue and the degree of inflammatory cells from the region of the artery. In variations in which an index of restenosis is determined, the system may display the index of restenosis for the region. For example, the device display may be configured to overlay an indicator of the index of restenosis for the region over a view including the region of the artery.
Also described herein are systems for indicating an enhanced risk of restenosis in an arterial tissue. For example, a system may include: an imaging modality configured to image a region of arterial tissue; and a processor configured to receive the image of the region of arterial tissue from the imaging modality and to determine a measure of hypercellularity and further configured to determine one or both of: a measure of how lipid-rich the tissue region is and a measure of how many inflammatory cells there are associated with the tissue region; and index logic configured to determine an index of restenosis for the tissue region based on the measure of hypercellularity and one or both of the measures of how lipid-rich the first tissue region is and the measure of how many inflammatory cells are associated with the first tissue region. The system may also include an output configured to output the index of restenosis.
As mentioned above, in some variations of the system, the index logic is configured to determine an index of restenosis based on the measure of hypercellularity, the measure of how lipid-rich the first tissue region is, and the measure of how many inflammatory cells are associated with the first tissue region.
Methods of treating atherosclerosis based on an estimate of the risk of restenosis as described herein are also provided. Also taught are methods, devices and systems for determining an enhanced risk of restenosis in an arterial tissue, as well as methods, devices and systems for treating and/or preventing restenosis in an arterial tissue.
For example, described herein are methods of determining an enhanced risk of restenosis in an arterial tissue. In some variations, these methods include the steps of: determining a measure of hypercellularity in a first arterial tissue region; determining one or both of: a measure of how lipid-rich the first tissue region is and a measure of how many inflammatory cells there are associated with the first tissue region; determining an index of restenosis for the first tissue region based on the measure of hypercellularity and one or both of the measures of how lipid-rich the first tissue region is and the measure of how many inflammatory cells are associated with the first tissue region; and presenting the index of restenosis for the first tissue region.
The step of determining an index of restenosis may include determining the index of restenosis for the first tissue region based on the measure of hypercellularity and the measure of how lipid-rich the first tissue region is and the measure of how many inflammatory cells are associated with the first tissue region.
The step of presenting may include displaying an image of the first tissue region with a visual indicator of the index of restenosis. In some variations, the method further includes imaging the first tissue region with an imaging modality configured to detect hypercellularity and/or imaging the first tissue region with an imaging modality configured to detect lipid-rich regions. In any of the devices, system and methods described herein, a measure of hypercellularity may be determined using an imaging modality such as optical coherence tomography to image the arterial tissue or a region (e.g., the “first region”) of the tissue.
The step of determining a measure of hypercellularity may include counting or estimating the amount of satellite-to-spindle-shaped smooth muscle cells within stroma. In general, determining a measure, estimate or count of hypercellularity may include determining the density of cells (e.g., muscle cells) within the stroma or a region of stroma fibrotic stroma rich in proteoglycan materials). The step of determining a measure of how lipid-rich a tissue region is may comprise estimating the amount or degree of amorphous material containing cholesterol crystals, loosely aggregated necrotic debris and foam cells. The step of determining a measure of how many inflammatory cells are associated with the first tissue region may include counting or estimating clusters of macrophages and lymphocytes.
In any of the devices, systems and methods described herein, the arterial tissue may be treated with a marker, dye, or indicator, which may help in determining a measure/estimate/count of the degree of hypercellularity, lipid-richness and/or presence of inflammatory cells.
In some variations, the methods described herein may also include the step of inserting a stent adjacent to the first arterial tissue region when the index of restenosis indicates a greater likelihood of restenosis. Other treatment methods may be used as well. For example, tissue (additional tissue in some cases) may be excited, the arterial region treated locally with one or more drugs or therapies (e.g., ablated, heat-treated, etc.), or the like.
In some variations of the methods described herein, tissue (e.g., an arterial tissue region) may be removed from the patient before or during the procedure, including before or during the estimation of hypercellularity, lipid-richness or the presence of inflammatory cells. In some variations it is the removed tissue that is examined; in other variations in is the tissue left behind that is examined; while in still other variations both tissues are examined.
Also described herein are methods of preventing restenosis in an arterial tissue. For example, a method of preventing restenosis may include: determining an index of restenosis for a first arterial tissue region based on a measure of hypercellularity of the first arterial tissue region and one or both of a measure of how lipid-rich the first arterial tissue region is and a measure of how many inflammatory cells are associated with the first arterial tissue region; and inserting a stent adjacent to the first arterial tissue region when the index of restenosis indicates a greater likelihood of restenosis. As mentioned above, in some variations other methods of treating the artery may be used in addition to, or in place of, the insertion of a stent.
The method may further include removing of tissue from the first arterial tissue region, either before (to analyze) or after (to treat). In some variations, the step of determining an index comprises imaging the first arterial tissue region in real or near-real time.
Section I, below, describes the key observation that quantitative histology may be used to predict rates of restenosis in patients undergoing atherectomy. In particular, certain levels of hypercellularity may indicate restenosis. The degree of lipid-rich tissue, as well as the level of inflammatory cells in the tissue may also be combined (individually or together) with the level of hypercellularity or other factor to provide an indication (which may be provided as an index) of the likelihood of restenosis. Section II describes how these observations may be applied.
Section I: Quantitative Histology
In an initial study, patients with angiographic follow up data and with a good quality tissue sections for histological evaluation were used. A total 409 specimens from native, primary (de novo) coronary artery lesions, and 354 specimens from restenosis lesion with prior intervention (balloon angioplasty, directional atherectomy or both) were included for the analysis.
Tissue Collection, Process and Slide Scan
Atherosclerotic tissue fragments were removed from the collection chamber of atherectomy catheter and fixed in 10% buffered formalin, processed through graded alcohols, and xylerte, and embedded in paraffin. Tissue sections of 4-6 um thick were cut and stained with hematoxylin and eosin, Masson's trichrome, and elastic van Gieson stains. The stained slides were scanned into digital images using a slide scanner, e.g., ScanScope CS (Aperio, Vista, Calif. 92081).
Characterization of Atherectomy Tissue Specimens
Various histological elements or components were described as follow:
Hypercellular: Hypercellular plaque tissue was characterized by the presence of numerous satellite-to-spindle shaped smooth muscles cells within loose-to-mildly fibrotic stroma rich in proteoglycan materials (see, e.g.,
Fibrocellular: Fibrocellular plaque tissue was consisted of moderate amount of connective tissue and intermediate numbers of smooth muscle cells (
Fibrous: Fibrous plaque tissue was defined by presence of abundant dense connective tissue with sparse cells (
Lipid-rich: Lipid rich lesion was defined as an area of amorphous materials containing cholesterol crystals, loosely aggregated necrotic debris or collection of foam cells (
Inflammatory cells: Inflammatory cell infiltration was evidence by the presence of clusters of macrophages and lymphocytes (
Thrombus: Thrombus was defined as an organized collection of fibrin, platelets and red blood cells (
Hemorrhage: Hemorrhage was defined as collections of erythrocytes within plaque matrix that were outside of vasa vasorum and that resulted in some distortion of the plaque structure (
Media: Media was recognized by the presence of internal elastic membrane and more orderly smooth muscle cells and connective tissue matrix (
Adventitia: Adventitia was defined as a vessel layer consisted of coarse fibrous connective tissue bundles with fragments of external elastic membrane, and some times, admixed small blood vessels or nerves (
Evaluation and Quantification of Histological Elements Atherosclerotic Plaque Tissue in Digital Images
The digital images were reviewed to define different histological components in the section. ScanScope computer analysis tools were used to draw boundaries around each tissue fragment and measure total section area on the digital slide (
Quantitative Histology and its Clinical Relevance
The quantitative histology data were combined with clinical and angiographic follow-up information to analyze the relation between individual histology component and clinical outcome after directional atherectomy procedure.
Analysis
Tissue taken from all of the 825 patients (approximately 4000 specimens) was examined as described above. The analysis was performed without any knowledge of the patient outcomes. As part of the analysis, the criterion above were used to quantify the areas of cellular hyperplasia, media, media and adventitia, thrombus and hemorrhage, lipid and inflammatory cells, unidentified fibrocellular, and fibrous tissue, by individually inspecting and drawing the area around each component on over 4000 specimens. The total section area was measured by computer and these values were used to calculate the individual percentages for each component. A summary of the measured components appears in Table 1, below. All variables ending with mm2 represent the area measurements in square mm while variables ending with area are expressed as percentages of the total section area (for example, for the 825 slides available the square mm of fibrous area (fibareamm2) averaged 3.18 mar and the total section area (totalsectionmm2) averaged 9.70 mm2 so 33.3% of the total section was fibrous tissue as determined by quantitative histology using this system.
These histological results were matched using the DCA procedure number on the tissue slides with the DCA number on the follow-up records, and merged. The resultant database was used to determine if there were any histological predictors for risk of restenosis in the population combining de novo and restenosis lesions. The analysis was repeated for patients who had not had a previous procedure (de novo lesions) and repeated for those patients who had been previously treated (restenosis lesions.).
As expected the best predictor of reduced risk of restenosis was the post interventional minimal lumen diameter (UM). The larger the lumen that was achieved at the end of the intervention the lower the restenosis rate (Baim and Kuntz bigger is better theory).
For the 825 patients with saved slides, clinical and follow-up quantitative angiography was available for 692 (83.3%) of the patients. Using QCA the angiographic restenosis rate was 39.6% (all pts), 37.5% (de novo pts) and 42.0% (restenosis pts).
Univariant analysis using Student's t-test showed that there was an increased incidence of restenosis in de novo lesion comparing the presence or absence of hypercellular plaque measured quantitative histology. For de novo patients with hypercellular plaque present in the histology the restenosis rate was 45% vs. 30% when hypercellular plaque was absent. P=0.0019. This association became even more pronounced when lipid and inflammatory cells were present. In patients with de novo lesions that had both hypercellular plaque as well as lipid and inflammatory cells the restenosis rate was 50% compared to 28% when both lipid/inflammatory cells and hypercellular plaque were not present.
Stepwise logistic regression was then used to compare MLD post intervention to the quantitative histological parameters seeking to determine if any of the histology findings were independent predictors of restenosis in the de novo patient population. MLD post (p=0.000) and hypercellularity expressed as a % of total section area (p=0.012) were both independent predictors of restenosis. The % of tissue represented by media/adventitia (p=0.317), lipid/inflammatory cells (p=0.881) and thrombus/hemorrhage (p=0.394) were not independent predictors of restenosis, as indicated in Table 2, below:
When the analysis was repeated for those de novo patients with both lipid/inflammatory cells and hypercellularity the predicative value of quantitative histology increased, Step-wise logistic regression showed the relationship between quantitative histological evidence of hypercellularity and restenosis at 6-9 month follow-up to be more significant for both MLD post and hypercellular % area (p=0.001 for both), as illustrated in Table 3.
These findings confirm that MLD post was an independent predictor of restenosis in the de novo patient population (as expected). However, the finding that quantitative histology provides a new parameter as an independent predictor of restenosis is surprising. When quantitative histology confirms the presence of both hypercellularity and lipid/inflammatory cells, this combination is as powerful as MLD post as an independent predictor of restenosis. Unexpectedly, quantitative histology may provide a new parameter as an independent predictor of restenosis. Based on these findings, when quantitative histology confirms the presence of both hypercellularity and lipid/inflammatory cells, this combination is as powerful as MLD post as an independent predictor of restenosis.
This new finding is not dependent on classical histological techniques, such as those used above. Using light microscopy and routine histological staining may take several days and may be of limited value in helping drive decisions on patient treatment during an actual procedure. Thus, described briefly in Section II below are systems for providing real-time tissue characterization with the resolution approaching that of light microscopy that allow or provide tailored therapies directed toward the biology of the lesion. For example, in some variations, Optical Coherence Tomography may be used, although the general methods and applications described herein are not limited to any particular modality.
Section II: Applications
A system (e.g., a system for treating atherosclerosis) may be provided that is configured to allow visualization (direct imaging) or an indicator of one or more of any of the factors described above. In a particular, a system may be configured to provide visualization or an indication of hypercellularity, lipid-rich tissue regions, and/or inflammatory cells. In some variations the system may provide an index of one or more of these factors, or a “restenosis index” based on one or more of these factors. In some variations, the system may provide an image of a tissue region (e.g., a peripheral vessel) that allows visualization of one or more of hypercellularity, lipid-rich tissue and/or inflammatory cells. The system may be configured so that multiple versions of the same image are displayed that are specific for showing one or more of these factors. The system may also include logic that assists the user in identifying or quantifying these factors.
In one example, a system for treating atherectomy includes one or more visualization modalities that permit visualization one or more of these factors. For example, an optical coherence tomography (OCT) imaging modality may be used. OCT may therefore provide real-time data indicating, for example, multicellularity, lipid content and/or inflammatory cells. An OCT system may be configured to use one or more wavelengths of light (or a band or mixture of wavelengths) that is selective for one or more of these features. Any of the imaging systems described herein (including OCT) may be used in conjunction with one or more markers (e.g., vital dyes, contrast agents, etc.) to help visualize. In some variations, the OCT may be used in vivo prior to excising the tissue. In other variations, the tissue may be examined as (or shortly after) it is removed from the vessel. Thus, any of the systems described herein may include an atherectomy device such as an atherectomy catheter. In some variations, the catheter may be guided or controlled based in part of the feedback or guidance from the determination/visualization of one or more of the factors described herein. For example, regions of the tissue exhibiting hypercellularity may be excised more completely or aggressively than other stenotic regions, or may be treated by stenting and/or the application of a local drug agent.
Preliminary analysis of human cadaver coronary artery tissue by OCT compared to a routine light microscopic image of the same vessel at the same site suggests that OCT may be configured to distinguish the lipid and fibrous components. OCT variations that may be used include OCT systems having multiple fibers, polarization OCT imaging, multiple/selectable wavelength, birefringence imaging using OCT, combinations of OCT imaging with ultrasound or other tissue-perturbation techniques, or the like. For example, OCT may be used to examine the elastic properties of the tissue which may correspond to the lipid content. Perturbing (e.g., vibrating) the tissue either directly (mechanically by pushing against the tissue, including inflating a balloon against a region of the tissue and imaging it) or using ultrasound (to vibrate the tissue) may indicate the lipid composition of the tissue region.
For example,
Other imaging modalities that may be used with the systems described herein, either alone or in combination, may include ultrasound, angiography (e.g., QVA), CT, MRI, SPECT, PET/CT, X-ray, etc. Virtually any imaging modality may be used, particularly those that may provide images of vessel regions displaying hypercellularity, lipid-rich tissue, and/or inflammatory cells.
Indication of the hypercellularity, lipid rich tissue, inflammatory cells and/or other factors may be provided in real time, near-real time, or otherwise during the procedure, as mentioned above. “Near-real” time may refer to a slight delay (e.g., time delayed images) compared to strict real time; for example an image in near-real time may lag by a few seconds or minutes. In some variations images illustrating the stenosed tissue regions may be saved for later analysis. In still other versions the tissue may be removed before the analysis, and correlated with a particular region, or merely with a particular patient. For example, an atherectomy device may be used to remove the tissue, which can then be examined (including by staining, fixation, or other treatments not typically advocated before removal from the patient) for these factors.
Any of the systems described herein may be configured to provide automated analysis of these factors. For example, a system for treating atherosclerosis may include logic for analyzing images of the vessel and determine an index of one or more of hypercellularity, lipid-rich membrane, and/or inflammatory cells. An index may be quantitative (e.g., a percentage, or percentage area, or square or cubic area or density). The index may be qualitative (e.g., “high”, “medium”, “low”, etc.). An index for the risk of restenosis may also be provided, based on the predictive risks described above. For example, an index of restenosis may be provided based (weighted heavily) on the degree or extent of very active (e.g., hypercellularity) tissue when there is a significant increase in lipid-rich tissue and/or inflammatory cells. Thus, in some variations, the system may include image analysis logic configured to examine one or more of the features described above.
Logic (e.g., indexing or detecting logic) may include computer-executable code (software), hardware, firmware, or any combination of these. For example, detection and/or index logic may be executable on or as part of a computer processor (e.g., microprocessor) that is either a general-purpose processor, a distributed processor, or a dedicated processor (or processors).
In some variations the system provides images that are colored, highlighted, or otherwise marked to indicate regions displaying some threshold (typically correlating to an enhanced risk for restenosis) based on one or more of the factors described herein. Multiple images may be displayed and/or marked, Or a single composite (e.g., “high risk” for restenosis) image may be provided.
Also described herein are methods of determining a risk of restenosis and methods of treating atherosclerosis.
In general, a method of determining a risk of restenosis as described herein may include the steps of determining from the tissues of a vessel if the tissue is hypercellular. The method may also include determining if the tissue is lipid-rich and/or the extent of inflammatory cells in the tissue. Determining if the tissue is hypercellular, lipid-rich and/or the extent of inflammatory cells may include determining a quantitative measure of the extent of hypercellularity, lipid-rich tissue and/or the extent of inflammatory cells. The tissue may be visualized and these determinations may be made by a visual means, or the determinations may be made without presenting an image of the tissue.
Determining if a tissue is hypercellular may also include determining the density of cells per unit area, or the density of a marker for cells (e.g., nuclei, cell membranes, etc.). As mentioned above, a determination of hypercellular tissue may mean simply presenting an image of the tissue in a modality that allows visualization of hypercellular tissue. For example, determining if a tissue is hypercellular may mean displaying an OCT image taken with a wavelength or plurality of wavelengths that permit visualization of hypercellularity (or a birefringent image, a polarized OCT image, etc.). Regions of relative hypercellularity may be marked or unmarked on the image. Similarly, determining if a tissue is lipid-rich may mean simply displaying an image of tissue that shows the relative lipid-richness of the tissue, which may be marked or unmarked on the image; determining the extent of inflammatory cells may mean showing an image of a tissue in which it is possible to detect inflammatory cells (or one or multiple types).
In some variations, the determination steps described may include adding a marker, dye, or indicator of the factor to be evaluated (e.g., cellularity, lipid content, inflammatory etc.). The determining step may also include perturbing the tissue so that the factor to be evaluated may be more readily determined using a particular methodology that benefits from this perturbation (e.g., by changing the temperature of the tissue, by vibrating the tissue, by irradiating the tissue, etc.).
For example, in
Methods of determining a risk of restenosis may also include determining an index of restenosis based on the determination of one or more of the factors mentioned herein, including hypercellularity, lipid content, and/or inflammatory cells. In some variations the index may be presented for the patient as a whole (a global index) or for specific regions mapped to the patients anatomy (e.g., within the vessels). Thus, a method of determining a risk of restenosis my be present as an image or series of images of the subject's vessel lumen, indicating regions of greater and/or lesser risk. Any of the imaging modalities described herein may be used in the determining steps mentioned above.
In some variations, the methods of determining the risk of restenosis may also include the step of inserting a device configured to help determine the risk of restenosis (e.g., a catheter, probe, etc.) within the vessel. Alternatively, in some variations, the method may include determining the risk non-invasively, using one or more imaging modalities from outside of a patient.
As mentioned, any of the methods described herein typically include the step of determining if a tissue (e.g., peripheral vascular tissue) is one or more of hypercellular, lipid-rich and/or includes inflammatory cells. Any of these determining steps may also include determining the extent to which the tissue is hypercellular, and/or includes in inflammatory cells. For example, a measure of hypercellular, lipid-richness and/or density of inflammatory cells may be compared to a standard or metric for these factors, based on the experimental data described above. The measure may be +/− some percentage of a threshold value (e.g., within +/−1%, 2%, 3%, 5%, 10%, 15%, 20%, 25%, 30%, 50%, etc. of a threshold value indicated from the experimental data).
A method of treating atherosclerosis typically includes the step of determining if a tissue (e.g., peripheral vascular tissue) is one or more of hypercellular, lipid-rich and/or includes inflammatory cells as mentioned above. This (these) determining steps may include any of the variations described above. The method of treating atherosclerosis may also include the step of removing tissue from the vessel. This removing step may be performed before, during or after the determining step(s).
In some variations, the method of treating atherosclerosis also includes the step of treating regions of the vessel that have a higher risk for restenosis (as suggested by the determination of one or more of hypercellularity, lipid richness and/or inflammatory cells) more aggressively than regions of lower risk. For example, regions of de novo atherectomy lesions having a higher hypercellularity and/or risk of restenosis may be treated with a drug eluting stent while atherectomy alone or atherectomy with a bare metal stent could be advised for less cellular lesions.
In some variations, the method of treating atherosclerosis may include the step of providing a pharmacological agent if it is determined that the subject is at greater risk for restenosis. For example, based on a subject's overall risk of restenosis, the subject may be given anticoagulants (e.g., clopidogrel (Plavix), etc.), or drugs that prevent excessive cell division (e.g., within the lumen), or the like.
The data describe above may also be interpreted to suggest that good results may be achieved by getting the best possible luminal gain with any intervention (atherectomy, stent, etc.) even to the extent of resecting media and adventitia with atherectomy, as long as the vessel is not perforated. Media and adventitia in the quantitative histology was not associated with an increased risk of restenosis, and a trend toward reduced restenosis was seen when media was present (p=0.107) in the extracted tissue. These data may support the concept that the cellularity of a de novo lesion is an important predictor or restenosis intervention. Thus any of the methods described herein that could maximize luminal gain, avoid perforation, and characterize the underlying tissue would be very desirable to reduce restenosis, either locally (e.g., at regions of greater risk for restenosis or in patients at higher risk) or globally. Overall a determination of the risk of restenosis may be useful to help guide the aggressiveness of the treatment.
The examples and illustrations included herein show, by way of illustration and not of limitation, specific embodiments in which the subject matter may be practiced. Other embodiments may be utilized and derived there from, such that structural and logical substitutions and changes may be made without departing from the scope of this disclosure. Such embodiments of the inventive subject matter may be referred to herein individually or collectively by the term “invention” merely for convenience and without intending to voluntarily limit the scope of this application to any single invention or inventive concept, if more than one is in fact disclosed. Thus, although specific embodiments have been illustrated and described herein, any arrangement calculated to achieve the same purpose may be substituted for the specific embodiments shown. This disclosure is intended to cover any and all adaptations or variations of various embodiments. Combinations of the above embodiments, and other embodiments not specifically described herein, will be apparent to those of skill in the art upon reviewing the above description.
This patent application claims priority to U.S. Provisional patent application Ser. No. 61/267,811, filed on Dec. 8, 2009, titled “DEVICES AND METHODS FOR PREDICTING AND PREVENTING RESTENOSIS”, which is herein incorporated by reference in its entirety.
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