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1.IntroductionWith an estimated 22,240 newly diagnosed cases and 14,030 deaths in the United States in 2013,1 ovarian cancer remains one of the most enigmatic cancers. Although the 5-year survival for patients with the disease detected at an early, localized stage is 92%, the overall 5-year survival for all women diagnosed with epithelial ovarian carcinoma is only 44% due to poor prognosis when diagnosed at a late stage. Unfortunately, 85% of ovarian cancers are detected at a more advanced stage as symptoms are easily missed until the disease has spread to other regions of the body.1 The disparity in survival rates between early and late stage ovarian cancer is due largely to the lack of appropriate screening techniques for asymptomatic, low risk population and inadequate sensitivity and specificity of existing screening methods for high risk women.2–4 Due to overall high mortality of ovarian cancer, women at elevated risk may be counseled to undergo prophylactic and, possibly unnecessary, oophorectomy. A sensitive, minimally invasive monitoring method could be used to preserve fertility in this subset of women. There are two potential advantages of developing an optical imaging approach for the ovaries, fallopian tubes, and peritoneum in this context. First, women at elevated risk for the development of this disease are frequently counseled to undergo prophylactic, salpingo-oophorectomy at an early age resulting in early surgical menopause with accompanying poor quality of life. In this case, an alternative sensitive and minimally invasive monitoring method has the potential to be impactful. Second, once early ovarian cancer is suspected in a young woman, a small subset of cases, there is the potential of preserving future reproductive capacity and endogenous hormonal function. For this group of patients, a sensitive and specific intraoperative means to detect metastatic disease to the other ovary could be helpful adjuvant to standard of care surgical staging, combined with preoperative transvaginal ultrasound with or without computed tomograpy (CT) scan. Intraoperative optical imaging enables examination of intraperitoneal surfaces at a higher resolution than the gold standard transvaginal ultrasound due to the use of light instead of oscillating sound waves and improved access to all peritoneal surfaces. Examination of the ovary and fimbrial surfaces is of particular importance as up to 90% of ovarian cancers are epithelial carcinomas and arise from either the ovarian or fimbrial epithelium.5–7 Traditional white-light laparoscopy provides reliable surface imaging for the detection of larger ovarian neoplasm; however, early cancer development involves microscopic alterations of tissue structure, and subsurface transformations to the ovarian stroma, indicative of a nascent tumor microenvironment.8 High resolution, subsurface laparoscopic optical imaging of epithelial and stromal microarchitecture could potentially reveal a developing neoplasm that would otherwise be missed by a surgeon making the critical decision to either remove or leave the ovaries. To optically visualize changes in surface epithelium and the subsurface stroma in carcinomas, several optical imaging modalities have been investigated, including optical coherence tomography (OCT),9–11 confocal microscopy,12 multiphoton microscopy,12–17 and reflectance spectroscopy and microscopy.18–22 OCT provides relatively large imaging depth and high temporal resolution, however it requires scanning and image reconstruction, adding to the complexity and cost of the instrument. Confocal microlaparoscopy demonstrates high spatial resolution, but requires raster scanning, restricting the ability to image multiple depths quickly. Multiphoton microscopy, including two-photon excitation fluorescence, second-harmonic generation (SHG), and third-harmonic generation (THG), has shown promise for detecting structural and metabolic differences between normal and abnormal tissues. In particular, SHG of collagen and THG of cell nuclei can provide tissue and cell morphological information in vivo that would otherwise only be accessible ex vivo by traditional hematoxylin and eosin (H&E) staining of fixed histological tissue sections.15–17,23,24 Although promising for visualizing early changes indicative of cancer, multiphoton imaging methods rely on raster scanning and require a complex laser source. Alternatively, multiplexed volume holographic imaging, which can be realized in a mechanically simple, robust, and inexpensive system, allows for imaging of multiple depths simultaneously.25 Should the cost and technical challenges of in vivo OCT, confocal, or multiphoton imaging be overcome, adjunct volume holographic imaging for close examination of suspicious regions could be beneficial. The volume holographic imaging system (VHIS) that we present here uses a multiplexed volume hologram and inexpensive light sources to achieve depth selectivity and background rejection. This VHIS is capable of both epireflectance and epifluorescence imaging at two imaging planes with lateral and axial resolutions of approximately 4 and 22 μm, respectively.26 We believe this to be the first demonstration of using a multiplexed volume hologram for imaging into highly scattering tissue such as the ovary. Although traditional optical microscopy or microlaparoscopy provides high quality images from a single, in-focus object plane, holographic imaging allows simultaneous acquisition of images from multiple planes within a three-dimensional volume. The resulting images from each depth plane are displayed side-by-side on a two-dimensional (2-D) monitor. The ability to simultaneously capture multiple reflectance or fluorescence images at depth within a volume of tissue is enabled by the multiplexed volume hologram, previously described by our group.27–29 The hologram is recorded by exposing a photosensitive polymer, 1,9-phenanthrenequinone-doped poly(methyl methacrylate) (PQ-PMMA), to an optical interference pattern formed with coherent laser illumination. To multiplex, a separate hologram is recorded into the same region of the element that will select light from a separate depth within the tissue sample. Upon illumination of the sample, light originating from each depth is collected by the different holograms and mapped to distinct regions on the detector without overlap. If illuminated by a narrow spectral bandwidth, as from a laser, a vertical line image is formed. If instead broadband illumination is used, or if fluorescence emission from the tissue sample is generated, a continuous series of adjacent line images are formed (along the -axis) according to the Bragg matching relation,30 producing a lateral field of view (FOV) that is proportional to the spectral bandwidth of the source. In the orthogonal direction (-axis), spectral Bragg matching condition is degenerate and the FOV is dictated by the imaging optics relation as in a conventional microscope. For the experiments presented in this paper, two images from two tissue depths are used; however, in earlier work, five depth projections were demonstrated, but it is possible to increase the number of depth projections beyond this with different system geometries.29 Targeted fluorescent probes that selectively bind to cancer cells over normal cells have shown promise for delineating cancer boundaries and improving outcomes of optical imaging-aided cytoreductive surgeries.31,32 We have previously demonstrated fluorescence VHIS imaging using fluorescent agents that are tailored to the spectral range detectable by the VHIS.27 In this study, we demonstrate fluorescence-mode volume holographic imaging alongside the primary reflectance-mode imaging of gynecological tissues provided by the fluorescent agents with emission spectra that fall within the same spectral range as the reflectance light source. We examine for the first time the performance of VHIS in video-rate imaging of surface and subsurface morphologies on a wide range of human ex vivo ovarian tissues collected during bilateral salpingo-oophorectomy (BSO), hysterectomy with bilateral salpingo-oophorectomy (H-BSO), total abdominal hysterectomy with bilateral salpingo-oophorectomy (TAH-BSO), and debulking surgery. To complete this study, we fabricated a benchtop VHIS specifically for ex vivo tissue imaging; however, the system is configured for rapid adaptation into a handheld endoscope for future in vivo imaging studies of gynecologic tissues. Although laparoscopic screening is likely unsuitable for routine screening of average risk women, in the cases of exploratory laparotomy of symptomatic women, or screening of high risk women, laparoscopic VHIS imaging could improve the specificity when determining the necessity of prophylactic salpingo-oophorectomies, possibly reducing the unnecessary ovary removal, and therefore improving the quality of life. 2.Materials and Methods2.1.PatientsTwenty-eight patients undergoing BSO, H-BSO, TAH-BSO, or debulking surgery at University of Arizona Medical Center—University Campus in Tucson, Arizona were asked to participate in this ex vivo tissue imaging study that spanned 9 months. The study was approved by the Institutional Review Board of the University of Arizona and informed consent was obtained from each patient who participated. Two consented patients were omitted from the study due to limited availability of tissue discards. From the 26 remaining patients included on this study, 118 tissue discard specimens were acquired for examination by VHIS. 2.2.Volume Holographic Imaging SystemThe benchtop VHIS used for this ex vivo tissue study was designed with a multiplexed hologram comprising two separate holograms within this single element, configured for imaging two planes in surgical biopsies, and displaying each side-by-side on the camera, as described in Fig. 1. Specific technical details on fabrication and use of multiplexed volume holographic imaging are thoroughly described in the previous works by our group and other groups.23,26,33–40 One hologram selects an image from the focal plane of the objective lens (similar to normal operation of a standard microscope) and the second hologram captures the defocused wavefront image originating from 50 μm above the focal plane. Each object wave was recorded with a different reference beam angle to provide side-by-side projections onto the detector—the in-focus depth image to the right half and the defocused wavefront image to the left half. The 50 μm separation between images was determined by the hologram construction parameters and the center wavelength of the reflectance light source (695 nm), and the FOV is determined by the spectral bandwidth. For this ex vivo tissue imaging study, the source’s 55-nm bandwidth corresponded to a 160 μm FOV along the -axis of the image. To enable rapid switching between reflectance and fluorescence imaging, the reflectance LED source was chosen with a central wavelength coinciding with the peak emission wavelength from the fluorescent dyes. A long-pass filter with 665 nm cut-on wavelength was used for both reflectance and fluorescence operation, acting to suppress the laser excitation in fluorescence mode. A schematic and photograph of the benchtop VHIS are shown in Figs. 2(a) and 2(b), respectively, depicting the system’s key components. The interchangeable illumination consists of either a 690 nm broadband LED (H2A1-H690, Roithner Lasertechnik GmbH, Vienna, Austria) for reflectance imaging or a 635 nm laser diode (BWF, B&W Tek, Incorporated, Newark, Delaware) for fluorescence imaging. In either scheme, illumination light passes through a pellicle beam splitter (BP150, Thorlabs Incorporated, Newtown, New Jersey) and then enters the , 0.55 numerical aperture (NA) objective lens with a 3.64-mm focal length (ULWDMSPlan50, Olympus America Incorporated, Center Valley, Pennsylvania). A Köhler illumination configuration is used to provide uniform illumination at the sample. Optical relays are used to project the pupil to the hologram plane which prevents beam shifting and signal loss. Reflected or fluorescent light originating from the sample is captured by the objective lens, redirected by the pellicle beam splitter, and filtered by the 665 nm long-pass filter (ET665LP, Chroma Technology Corporation, Bellows Falls, Vermont), which blocks the 635-nm excitation illumination in fluorescence mode, and reaches the multiplexed volume hologram. Here, the hologram diffracts and disperses the light along the -axis of the image. The multiplexed gratings in the hologram are designed to select light from the tissue surface and 50 μm below the surface. The light from these two channels is focused by a camera lens (AC254-075-A, Thorlabs Incorporated, Newtown, New Jersey) and projected side-by-side onto a CCD camera (ORCA-R2, Hamamatsu Corporation, Middlesex, New Jersey). VHIS images were acquired using HCImage Live software (Hamamatsu Corporation, Middlesex, New Jersey). The position of the tissue specimen is adjusted using a three-axis micropositioning stage (460A Series, Newport Corporation, Irvine, California) with a digital micrometer head (DM713, Thorlabs Incorporated, Newtown, New Jersey) for -axis control. As assembled, the VHIS provides lateral resolution of approximately 4 μm and an axial resolution of approximately . Future adaptation into a clinical endoscopic VHIS for in vivo imaging will be achieved by replacing the objective lens with a high NA endoscope and incorporating the hologram and all other optical components into a sealed handle for use by the oncological surgeon. 2.3.Tissue ImagingBiopsies (approximately 125 to ) were obtained from surgical discards and washed in phosphate-buffered saline (PBS) for up to 30 min following acquisition, followed by incubation in PBS containing fluorescent cellular markers for 30 min. The markers included a nuclear dye that permeates cell membranes and intercalates with deoxyribonucleic acid (HCS NuclearMask™ Deep Red Stain, Life Technologies Corporation, Grand Island, New York), and/or a membrane dye that selectively labels lipid bilayers (Vybrant® DiD Cell Labeling Solution, Life Technologies Corporation, Grand Island, New York). The peak excitation and emission wavelengths for the dyes were around 640 and 670 nm, respectively. These dyes were selected because of their emission spectra falling within the 665 to 720 nm designed dispersive axis of the VHIS. Specimens were briefly rinsed in PBS to remove excess dye prior to careful placement in a Petri dish for handling, ensuring exposure of the epithelial surface. To image with the VHIS, the sample was placed on the sample stage and brought into focus by adjusting the position of the stage in relation to the objective lens. To prevent drying, samples were hydrated with PBS while imaging. With the broadband LED illuminating the sample, reflectance images were acquired with the CCD camera set to binning for a final image dimension of . This allowed for continuous image acquisition at 10 to for 30 to 120 s while translating the stage laterally to scan a large area of the tissue specimen, mimicking conditions that would be used for in vivo laparoscopic imaging. For fluorescence-mode imaging, the illumination source was changed to the 635 nm laser diode and the camera was set to binning for a final image dimension of , allowing image acquisition at up to , similarly for 30 to 120 s. For the binned images, the apparent pixel size as mapped to object space is 0.63 μm for binning, and 1.25 μm for binning, both of which are below the system lateral resolution of 2 to 4 μm as imposed by the hologram. All image data were saved as multipage, 16-bit tagged image file format (TIFF) files and examined alongside histological micrographs from corresponding tissue sections. All tissues were imaged within 120 min of excision. 2.4.Histology and Pathological EvaluationImmediately following VHIS imaging, tissues specimens were affixed to filter paper to maintain orientation and submerged in fixation media (HistoChoice®, Sigma-Aldrich, Incorporated, St. Louis, Missouri). Fixed tissues were dehydrated in ethanol, embedded in paraffin wax, microtome sectioned at 5 μm, and prepared on slides. Tissue specimen orientation was maintained so the resulting slides produced cross sectional views of the samples, i.e., perpendicular to the en face VHIS image plane. Slides were H&E stained in preparation for pathological evaluation. Histological specimens were interpreted by a pathologist independent of patient diagnosis. 2.5.Image ProcessingRaw VHIS images were processed to equalize contrast and brightness variation of the left and right channels, as shown in Fig. 3. In this method, raw TIFF images, i.e., 2-D intensity matrices, were split into left and right submatrices with equal FOV. For each channel matrix, background signal was removed by subtracting the minimum intensity value of the matrix from each pixel within that matrix. This sets the minimum intensity value of both the left and right matrices to zero, represented as and , respectively. The deeper imaging plane, , consistently provided a dimmer signal as compared to . To equalize the intensity histograms of the channels, the right channel matrix was multiplied by a scalar equivalent to the ratio of over , the intensity ranges of and , as follows: where is the new, equalized 2-D right channel matrix. Finally, is rejoined with to form the intensity equalized VHIS image. For display in publication, image intensity ranges were adjusted to 5% to 95% of the gray level range.3.ResultsOne hundred and eighteen tissue specimens from 26 patients (ages: 22 to 73 years, average: 49.5 years, median: 47 years) were successfully imaged with the VHIS in both reflectance and fluorescence modes. More than 70,000 reflectance-mode images and 35,000 fluorescence-mode images were acquired in total. Between one and nine tissue specimens originating from ovarian, uterine, fallopian, and/or peritoneal tissues were acquired from each patient and individually imaged following excision. Of these specimens, 64 samples originated from the ovary, 39 from the fallopian tube, five from the ovarian cancer metastases within the peritoneum, and 10 from the uterus. At the time of surgery, seven patients were classified as high risk and received prophylactic surgeries, four were diagnosed with ovarian cancer, and 15 with benign ovarian neoplasms or conditions. In most cases, both normal and abnormal tissue specimens were acquired from a single patient. Table 1 summarizes the imaged tissue specimens grouped by pathological findings. Table 1Summary of tissues imaged.
The primary focus of the study was to assess the reflectance-mode performance of the VHIS for imaging ovarian tissues. Therefore, reflectance and fluorescent images were analyzed separately. Analysis was qualitative in nature to identify distinguishing morphological features between diagnostic categories. For the ovarian tissues, the predominant tissue specimen groups examined by VHIS were normal ovary (39) and ovarian serous adenocarcinoma (10). Other, less commonly observed ovarian abnormalities included ovarian mucinous adenocarcinoma (1), benign mucinous cystadenoma (5), benign serous cystadenoma (1), and simple ovarian cysts (3). Additionally, four ovarian cancer metastases to the peritoneum were imaged. In consideration of experimental observations indicating that ovarian serous adenocarcinoma commonly arises from the fimbriated end of the fallopian tube for women at high risk,5,41,42 we also examined 39 tissue specimens originating from fallopian tube in this study, of which only one was cancerous (fallopian tube serous adenocarcinoma). Ten uterine tissue specimens were also collected and imaged in this tissue study, including three normal endometrium, four normal myometrium, and three endometrial adenocarcinoma. As stated previously, the goal of this study was to extract common features observable in VHIS images within each tissue group that can be linked to their diagnosis. Features typically identified to diagnose tissue specimens in H&E-stained histological slides were the basis for these observations; however, VHIS is a vastly different modality than typical histology. Primarily, contrast in VHIS reflectance images is provided by variations in scattering and absorption of the illumination light within the tissue, revealing morphological information. Instead, H&E-stained slides provide contrast from the chromophores H&E to highlight cellular and tissue structures to inform diagnosis. Additionally, VHIS imaging is performed en face at two depths, while histological slides are prepared from cross-sectional slices perpendicular to the VHIS imaging plane. In all subsequent example VHIS images, the left and right channels correspond to the surface and subsurface planes, respectively. 3.1.Normal OvaryVHIS images of normal, epithelialized ovary showed very consistent features. Regular, cobblestone appearance of the surface, or left channel image, was observed in these normal ovarian tissues as demonstrated in Fig. 4(c), consistent with a monolayer of cuboidal epithelium, as confirmed by histology in Fig. 4(a). The subsurface or right channel of the normal ovarian tissue [Fig. 4(c)], which imaged a plane within the stroma, commonly showed a repeating wavy pattern corresponding to the regularity of the dense, Type I stromal collagen, also confirmed by histology [Fig. 4(a)]. The regular cobblestone-like pattern was also observed in the fluorescence images [Fig. 4(e)], but most fluorescent signal was consistently observed in the right or stromal channel due to the configuration of the camera in the imaging system. In five instances of normal ovarian tissue, the cobblestone epithelium was lost, resulting in flat and featureless VHIS images. Histology revealed that these ovaries were de-epithelialized peri- or postoperatively, likely due to handling. 3.2.Ovarian Serous AdenocarcinomaOvarian serous adenocarcinoma, the most common ovarian cancer, is characterized by well-formed papillae, abnormally large epithelial cells with large nuclei arranged in a disordered pattern that have invaded the stroma. Morphological heterogeneity is commonly observed in ovarian serous adenocarcinoma with high variability in nuclear size. All of these features were easily identifiable in histology as depicted in Fig. 4(b). Reflectance-mode VHIS images of ovarian serous adenocarcinoma similarly showed a stark divergence from the normal ovarian images, as seen in Fig. 4(d). Both surface and subsurface imaging channels showed topographical features of irregular and variable pits and valleys consistent with histology. Fluorescence-mode images of ovarian serous adenocarcinoma [Fig. 4(f)] revealed a larger and irregular nuclei and membrane staining than those seen in normal ovarian tissues, again consistent with histology. 3.3.Mucinous AdenocarcinomaOvarian mucinous adenocarcinoma is less common than its serous counterpart and is characterized by disorderly stromal invasion, nuclear atypia, and mucin producing as seen in histology [Fig. 5(a)]. VHIS reflectance-mode images [Fig. 5(e)] show distinct morphological differences from the normal ovarian tissue at both surface and subsurface depths with a poorly organized structure. Fluorescence-mode images [Fig. 5(i)] also show this irregular organization of mucinous adenocarcinoma. 3.4.Mucinous CystadenomaMucinous cystadenoma, a benign abnormality, is identified by one or more cystic tumors filled with mucinous fluid lined by tall columnar epithelial cells, as seen in histology in Fig. 5(b). Corresponding reflectance- and fluorescence-mode VHIS images are shown in Figs. 5(f) and 5(j), respectively. Although columnar epithelium is difficult to identify in the VHIS images, the reflectance and fluorescence observed are neither as regular as normal ovarian epithelium nor as irregular as ovarian serous adenocarcinoma in appearance. 3.5.Serous CystadenomaSerous cystadenoma, also a benign abnormality, is classified by papillary architecture and moderate nuclear atypia, apparent in histology in Fig. 5(c). Unlike serous adenocarcinoma, serous cystadenoma does not exhibit stromal invasion. Corresponding reflectance- and fluorescence-mode VHIS images are shown in Figs. 5(g) and 5(k), respectively. The reflectance and fluorescence images show larger punctuate features that span both surface and subsurface channels and may correlate to the typical papillary nature of serous cystadenoma. 3.6.Metastases to the PeritoneumExtraovarian peritoneal metastases derived from primary ovarian carcinoma exhibit microarchitectural features including tufting, nuclear atypia, and micropapillae, as seen in histology in Fig. 5(d). Reflectance-mode VHIS image of a metastasis biopsy is shown in Fig. 5(h) and exhibits a smooth background appearance in both channels with an irregular pattern of punctuate surface features. Similarly in the fluorescence-mode image [Fig. 5(l)], bright punctuate fluorescence is also observed. 3.7.Normal Fallopian Tube FimbriaAs mentioned above, the fimbrial epithelium has been implicated as the epicenter of ovarian carcinoma development in recent studies and therefore potentially a critical region to examine for early detection. In addition to the ovarian tissues, we examined 39 tissue specimens originating from fallopian tube tissue, of which 23 were diagnosed as normal, four as normal with stripped epithelium, 11 with chronic salpingitis, and only one cancerous case of serous adenocarcinoma of the fallopian tube. Histology of normal fallopian tube [Fig. 6(a)] shows uniformly epithelialized fimbriae with clearly defined boundaries and a semiregular distribution of stromal cells arranged in a storiform pattern. VHIS imaging of the fallopian fimbria revealed a unique and consistent pattern in reflectance- and fluorescence-modes [Figs. 6(d) and 6(g), respectively] of a regular pattern similar to that observed in normal ovary, but with larger features and a deep furrowing pattern. Although specific features from VHIS images of fallopian fimbrial did not clearly correlate to histological morphology, the uniformity of the images suggest that we may actually peering onto many fimbriae slumped upon each other, a nonphysiological morphology induced by placement in the Petri dish for imaging. 3.8.Fallopian Tube Serous AdenocarcinomaOnly one cancerous abnormality involving the fallopian tube was identified in the form of fallopian tube serous adenocarcinoma, as shown by histology in Fig. 6(b). Much like serous adenocarcinoma of the ovary, this fallopian tube version is also characterized by invasive and complex papillary architecture with irregular and variable nuclei. The reflectance-mode VHIS image [Fig. 6(e)] revealed a vastly different architecture than the normal fallopian tube, with a generally smoother appearance with a small number of irregular features. Fluorescence-mode VHIS images [Fig. 6(h)] also showed some irregularity, however only a very low signal level was observed. 3.9.Chronic SalpingitisChronic salpingitis is defined as inflammation of the fallopian tube, often caused by repeated or persistent bacterial or viral infections or other constant perturbations of the fallopian tubes. This condition is characterized by blunted or fused fallopian fimbriae as seen in histology [Fig. 6(c)]. Both the reflectance- and fluorescence-mode VHIS images of chronic salpingitis [Figs. 6(f) and 6(i), respectively] show a lower frequency pattern than observed in normal fallopian tube which instead exhibits many delicate fimbriae. 4.DiscussionThe results of this ex vivo tissue study support the development of multiplexed volume holographic imaging for imaging surface and subsurface morphologies of ovarian, tubal, and other gynecologic tissues. The VHIS implementation described here is considered for adaptation for future in vivo preclinical microlaparoscopic imaging of surface and subsurface features. The most striking correlation in VHIS images and tissue diagnosis was seen in both the normal ovarian tissues and ovarian serous adenocarcinoma. Normal ovarian tissue consistently showed a regular morphology under both the reflectance and fluorescent imaging modes, similar to what was observed in histology. Characteristic features included a regular cobblestone appearance in the surface image (left channel), matching the regularity of a healthy epithelium, and a regular subsurface pattern corresponding to the regularity of the stromal collagen. The regular cobblestone pattern was also observed in the fluorescence images. In ovarian serous adenocarcinoma, the en face VHIS images were strikingly different than the normal ovarian tissues, with an irregular topography consistent with the irregularity of carcinoma growth and micropapillae. In fluorescence-mode images, larger and irregularly shaped cells with nuclear atypia were observed, characteristic of cancerous epithelial cells. Analysis of the fallopian tube was confounded by folding of the normal fimbria and by the limited number of fallopian tube cancers (one) included in this study. Future studies will specifically include VHIS imaging of normal fallopian tube and its discrimination from serous adenocarcinoma involving the tube. To determine the sensitivity and specificity of VHIS as a diagnostic tool for ovarian cancer, detailed examination of VHIS images, either computationally or by trained observers, will be necessary. Traditional histological analysis of tissue biopsies remains the gold standard for diagnosing ovarian cancer; however, the potential real-time information that laparoscopic VHIS provides to the oncological surgeon could help to inform in situ decisions to remove or preserve a patient’s ovaries more rapidly than waiting for histological results. A diagnostic laparoscopy with the VHIS may be useful for detecting cancer in normal-risk patients already undergoing exploratory laparotomy or laparoscopy, or for high-risk patients desiring regular laparoscopic screening with sensitive optical techniques as a short-term option to preserve fertility. Future quantitative analysis of VHIS images will likely elucidate the diagnostic capability of VHIS. We have previously shown that a variety of quantitative image analysis techniques can be useful for identifying diseased tissues.16,43 In particular, analysis of the spatial frequency spectrum and gray-level co-occurrence matrix parameters of OCT and SHG images has shown promise for automated, quantitative discrimination between normal and abnormal tissues. These techniques will be applied to VHIS images to assess their utility as quantitative methods discerning normal tissue from ovarian cancer. The addition of fluorescent contrast agents to the VHIS was demonstrated using commercially available fluorescent dyes that target the cell membrane or nucleus. Although this was performed to demonstrate the ability of the system in capturing fluorescent images, future directions point toward the use of targeted contrast agents to highlight abnormal patterns of receptor expression associated with cancerous cells and tissues, as previously demonstrated in vivo using fluorescein loaded liposomes targeted to the folate receptor.44,45 With VHIS, the hologram maps spectral and spatial information along the -axis, resulting in an image inherently weighted by spectral intensity distribution of light reaching the CCD camera. In the case of reflectance mode images, this distribution is determined by the spectrum of the broadband LED used for illumination which is nearly uniform, however rolls off along the edges leading to a narrowed FOV. Future versions of the VHIS will address this limitation by instead using a broader spectral band source in combination with a band-pass filter that corresponds to the spectral range observed with the hologram. For fluorescent mode imaging, the spectral–spatial mapping leads to an image that is intensity weighted by the shape of the fluorescence emission spectrum. With the fluorescent dyes used in the report, sharp emission peaks near 670 nm results in bright image features on the leftmost portion of each channel with rapid diminishing of fluorescence signal moving to the right, or long wavelengths. Unlike traditional fluorescence microscopy, where the signal represents the integral of fluorescence emission intensities within the entire spectral range captured through optical filters, VHIS fluorescence disperses the signal. To address this deficiency, alternative dyes with broader fluorescence spectra or holograms designed to disperse a narrower band of wavelengths could be added for future investigation. Alternatively, the fluorescence images could be divided by the fluorescent dye’s emission spectrum along the -axis to attempt to equalize the signal. To take advantage of dispersion of the fluorescence spectrum along the -axis in the VHIS images, the use of specialized fluorescent dyes that exhibit spectral shifts in response to local environmental changes, such as pH or oxygenation, could reveal useful information about suspect tissues. Channel-by-channel optical depth sectioning is important to clearly observe distinct morphological features at the surface and subsurface locations in the tissue. The hologram used in this study was fabricated with an imaging depth separation of 50 μm. The measured full width at half maximum of the axial point spread function at both of these depths was 22 μm. Upon observation of the reflectance VHIS images of gynecologic tissues, it is apparent that there is some crosstalk between channels. Work to suppress channel crosstalk is currently underway by combining highly selective volume holograms with structured illumination to increase depth selectivity.26,46 The image intensity that reaches the CCD camera in the VHIS is very low compared to the illumination source due to loss in the instrument optics (particularly from the beam splitter utilized to operate in the reflectance mode, attenuation in the tissue, and selectivity of the hologram. Nearly 95% of light is not Bragg matched to the hologram (i.e., it does not correspond to the desired imaging depths) and passes through hologram and is captured by the beam dump. We estimate that the final photon flux that reaches the CCD camera is 2 to 3 orders of magnitude less than the photon flux of the illumination light. However, as demonstrated by the images shown within, the signal falls within the dynamic range and sensitivity of the camera and allows frame rates up to 20 fps. For this benchtop trial, imaging was performed in the dark to keep background noise low and preserve signal-to-noise ratio appropriate for video-rate holographic imaging. A future adaptation of the system for use in exploratory laparotomy, a situation where turning off room lights would not be ideal, could be designed for near-infrared (NIR) illumination (above 800 nm) to avoid background contribution from ambient light. VHIS fluorescence imaging could be achieved by administering intravenous, intraperitoneal, or topical fluorescent agents that fluoresce in the NIR, such as FDA-approved indocyanine green (ICG). As we have previously demonstrated using the PQ-PMMA holographic polymer for imaging at wavelengths up to 1500 nm,47 ICG fluorescence imaging would be compatible with VHIS. 5.ConclusionWe have demonstrated the use of VHIS for imaging ex vivo ovarian tissue specimens, enabling qualitative discrimination of normal and abnormal tissues as confirmed by histology. The benchtop VHIS described here provided simultaneous en face visualization of two image planes, at the tissue surface and at a depth of 50 μm in the tissue, expandable up to five or more imaging planes with a volume hologram constructed under different parameters. As evident in the example images shown in this paper, VHIS is capable of both epireflectance and epifluorescence imaging. We specifically designed the benchtop VHIS for rapid adaptation into an endoscopic version for an in vivo clinical trial, achievable by simply replacing the objective lens with a custom endoscope, and encasing the optical components and volume hologram into a handheld tool. Because VHIS is constructed in a mechanically simple and robust fashion, as it does not require raster scanning or specialized light sources to operate, rapid translation into a durable clinical instrument is feasible. We believe that widespread adoption of an optical imaging modality like VHIS for clinical visualization of early stage ovarian cancer has the potential to reduce the mortality and preserve fertility in high risk women. The results from this study assessing VHIS for simultaneous surface and subsurface imaging of gynecological tissues are promising for future clinical application of an endoscopic VHIS. AcknowledgmentsThe authors thank Ray B. Nagle, MD, PhD for his expertise in histopathological analysis and interpretation at the Tissue Acquisition and Cellular/Molecular Analysis Shared Service Core (TACMASS), which is supported by the University of Arizona Cancer Center Support Grant from the National Cancer Institute (NCI) of the National Institutes of Health (NIH) under Award No. P30CA023074. Research reported in this publication was supported by the NCI of the NIH under Award No. R01CA134424. Additional support was provided by National Heart, Lung, and Blood Institute of the NIH under Award No. T32HL007955 and the National Institute of Biomedical Imaging and Bioengineering of the NIH under Award No. T32EB000809. The content is solely the responsibility of the authors and does not necessarily represent the official views of the National Institutes of Health. ReferencesAmerican Cancer Society, “Cancer Facts & Figures 2013,”
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