Your search keyword '"Salman Farshchi-Heydari"' showing total 13 results

1. AB-452672-4 POINT-BY-POINT PULSED FIELD ABLATION USING A MULTIMODALITY GENERATOR: COMPARISON WITH RADIOFREQUENCY ABLATION IN REMAPPED CHRONIC SWINE HEARTS

Author

Luigi Di Biase, jacopo Marazzato, Fengwei Zou, Aung N. Lin, Vito Grupposo, Jennifer Maffre, Salman Farshchi-Heydari, Tushar Sharma, Christopher Beekler, Andrea Natale, Sanghamitra Mohanty, Assaf Govari, and Xiaodong Zhang

Subjects

Physiology (medical), Cardiology and Cardiovascular Medicine

Published

2023

2. Development of 68Ga-labelled DTPA galactosyl human serum albumin for liver function imaging

Author

Roland Haubner, Christine Rangger, David R. Vera, Anna Helbok, Irene Virgolini, Daniel Putzer, and Salman Farshchi-Heydari

Subjects

medicine.diagnostic_test, business.industry, General Medicine, Endocytosis, Human serum albumin, chemistry.chemical_compound, chemistry, Biochemistry, Positron emission tomography, Diethylenetriamine, medicine, Radiology, Nuclear Medicine and imaging, Hepatic Asialoglycoprotein Receptor, Liver function, Desialylated Glycoproteins, Nuclear medicine, business, Receptor, medicine.drug

Abstract

Purpose The hepatic asialoglycoprotein receptor is responsible for degradation of desialylated glycoproteins through receptor-mediated endocytosis. It has been shown that imaging of the receptor density using [99mTc]diethylenetriamine pentaacetic acid (DTPA) galactosyl human serum albumin ([99mTc]GSA) allows non-invasive determination of functional hepatocellular mass. Here we present the synthesis and evaluation of [68Ga]GSA for the potential use with positron emission tomography (PET).

Published

2013

3. Staging of fibrosis in experimental non-alcoholic steatohepatitis by quantitative molecular imaging in rat models

Author

Robert F. Mattrey, Carl K. Hoh, Rohit Loomba, David R. Vera, Bernd Schnabl, David A. Brenner, Cynthia Behling, Claude B. Sirlin, and Salman Farshchi-Heydari

Subjects

Liver Cirrhosis, Male, Cancer Research, medicine.medical_specialty, Pathology, Chronic Liver Disease and Cirrhosis, Clinical Sciences, Molecular imaging, Gallium Radioisotopes, Gastroenterology, Oral and gastrointestinal, 030218 nuclear medicine & medical imaging, 03 medical and health sciences, 0302 clinical medicine, Fibrosis, Non-alcoholic Fatty Liver Disease, Internal medicine, Biopsy, medicine, Animals, Humans, Galactosyl-neoglycoalbumin, Radiology, Nuclear Medicine and imaging, Stage (cooking), Serum Albumin, medicine.diagnostic_test, business.industry, Animal, Liver Disease, Pentetic Acid, medicine.disease, Molecular Imaging, Rats, Disease Models, Animal, Kinetics, Nuclear Medicine & Medical Imaging, ROC Curve, Positron emission tomography, Liver biopsy, Disease Models, Molecular Medicine, Biomedical Imaging, 030211 gastroenterology & hepatology, Liver function, Steatohepatitis, Steatosis, business, Digestive Diseases

Abstract

Objectives The aim of this study was to test the ability of hepatocyte-specific functional imaging to stage fibrosis in experimental rat models of liver fibrosis and progressive NASH. Using ROC analysis we tested the ability of a functional imaging metric to discriminate early ( F1 ) from moderate ( F2 ) fibrosis in the absence and presence of non-alcoholic steatohepatitis, which has not been achieved by any modality other than biopsy. Methods Galactosyl Human Serum Albumin (GSA) was radiolabeled with the positron-emitter, 68 Ga, and injected (i.v., 45–95μCi, 1.5pmol/g TBW) into 44 healthy, 19 DEN-, and 22 CDAA-treated male rats. Quantification of liver function was achieved by calculating T90 , defined as the time for the liver to accumulate 90 percent of the [ 68 Ga]GSA plateau value. All livers were excised immediately after imaging and prepared for a "blinded" histologic examination, which included fibrosis and fat content scores. Two sets of fibrosis scores were recorded for all of animals. The dominant fibrosis stage was recorded as the "Dominant Pattern" score and the "Maximum Pattern" score was assigned if a smaller distinct region with a higher fibrosis score was observed. Results Animals with Dominant Pattern F0 – F1 liver fibrosis ( D − =39) demonstrated significantly ( P 68 Ga]GSA (2.40±0.52min) than those with moderate to advanced Dominant Pattern fibrosis F2 and F4 ( D + =26) (3.48±1.01min). ROC analysis ( F0 – F1 vs F2 – F4 ) produced an area under the binormal curve ( AUC ) of 0.867±0.045. Twenty-seven of the 65 rats had small regions with higher fibrosis scores. Six of these Maximum Pattern scores reclassified the animals from D − to D + . ROC analysis of F0 – F1 versus F2 – F4 rats without liver fat produced AUCs of 0.881±0.053 for the Dominant Pattern Score and 0.944±0.035 for the Maximum Pattern Score. Conclusions PET Functional Imaging of [ 68 Ga]GSA accurately discriminates early from moderate experimental fibrosis independent of steatosis grade. If validated in human studies, molecular imaging may emerge as a potential alternative to invasive liver biopsy.

Published

2016

4. Quadrature Detection of Ultrasound-Modulated Photons with a Gain-Modulated, Image-Intensified, CCD Camera

Author

David J. Hall, Salman Farshchi-Heydari, and Ulas Sunar

Subjects

Physics, Photon, genetic structures, Optical contrast, Ccd camera, business.industry, Ultrasound, eye diseases, Quadrature (astronomy), Optics, Ultrasound imaging, sense organs, Molecular imaging, business

Abstract

Acousto-optic imaging promises to provide in vivo images of optical contrast but with the superior spatial reso- lution of ultrasound imaging. Here we present novel quadrature detection of ultrasound-modulated photons with a gain- modulated, image-intensified, CCD camera. The additional detection of ultrasound-modulated fluorescence photons dem- onstrates potential for in vivo acousto-optic molecular imaging.

Published

2008

5. Preclinical Evaluation of Robotic-Assisted Sentinel Lymph Node Fluorescence Imaging

Author

Zhengtao Qin, David R. Vera, Michael A. Liss, Christopher J. Kane, Sean Hickey, Salman Farshchi-Heydari, and David J. Hall

Subjects

Fluorescence-lifetime imaging microscopy, Pathology, medicine.medical_specialty, Fluorophore, Robotic assisted, Clinical Sciences, Sentinel lymph node, fluorescent tilmanocept, sentinel lymph node mapping, Fluorescence, robotic-assisted surgery, Article, chemistry.chemical_compound, Clinical Research, Paraaortic lymph nodes, medicine, Animals, Radiology, Nuclear Medicine and imaging, Spectrometry, business.industry, Sentinel Lymph Node Biopsy, Robotics, body regions, Nuclear Medicine & Medical Imaging, Fluorescence intensity, Spectrometry, Fluorescence, chemistry, Biomedical Imaging, Lymph Node Excision, Lymph, Rabbits, Molecular imaging, Nuclear medicine, business

Abstract

UnlabelledAn ideal substance to provide convenient and accurate targeting for sentinel lymph node (SLN) mapping during robotic-assisted surgery has yet to be found. We used an animal model to determine the ability of the FireFly camera system to detect fluorescent SLNs after administration of a dual-labeled molecular imaging agent.MethodsWe injected the footpads of New Zealand White rabbits with 1.7 or 8.4 nmol of tilmanocept labeled with (99m)Tc and a near-infrared fluorophore, IRDye800CW. One and 36 h after injection, popliteal lymph nodes, representing the SLNs, were dissected with the assistance of the FireFly camera system, a fluorescence-capable endoscopic imaging system. After excision of the paraaortic lymph nodes, which represented non-SLNs, we assayed all lymph nodes for radioactivity and fluorescence intensity.ResultsFluorescence within all popliteal lymph nodes was easily detected by the FireFly camera system. Fluorescence within the lymph channel could be imaged during the 1-h studies. When compared with the paraaortic lymph nodes, the popliteal lymph nodes retain greater than 95% of the radioactivity at both 1 and 36 h after injection. At both doses (1.7 and 8.4 nmol), the popliteal nodes had higher (P < 0.050) optical fluorescence intensity than the paraaortic nodes at the 1- and 36-h time points.ConclusionThe FireFly camera system can easily detect tilmanocept labeled with a near-infrared fluorophore at least 36 h after administration. This ability will permit image acquisition and subsequent verification of fluorescence-labeled SLNs during robotic-assisted surgery.

Published

2014

6. Cold wall effect eliminating method to determine the contrast recovery coefficient for small animal PET scanners using the NEMA NU-4 image quality phantom

Author

Imre Lajtos, Áron Krisztián Krizsán, Salman Farshchi-Heydari, Magnus Dahlbom, Freddie Daver, László Balkay, David R. Vera, Peter Major, Jozsef Molnar, Miklós Emri, Judit Lantos, Carl K. Hoh, Gábor Opposits, Johannes Czernin, Lajos Trón, Attila Forgács, and István Jószai

Subjects

Radiological and Ultrasound Technology, Wall effect, Computer science, Image quality, Phantoms, Imaging, media_common.quotation_subject, Monte Carlo method, Orvostudományok, Klinikai orvostudományok, Imaging phantom, Cold Temperature, Feature (computer vision), Small animal, Positron-Emission Tomography, Contrast (vision), Animals, Radiology, Nuclear Medicine and imaging, Artifacts, Monte Carlo Method, Simulation, Biomedical engineering, media_common

Abstract

The contrast recovery coefficients (CRC) were evaluated for five different small animal PET scanners: GE Explore Vista, Genisys4, MiniPET-2, nanoScan PC and Siemens Inveon. The NEMA NU-4 2008 performance test with the suggested image quality phantom (NU4IQ) does not allow the determination of the CRC values for the hot regions in the phantom. This drawback of NU4IQ phantom motivated us to develop a new method for this purpose. The method includes special acquisition and reconstruction protocols using the original phantom, and results in an artificially merged image enabling the evaluation of CRC values. An advantageous feature of this method is that it stops the cold wall effect from distorting the CRC calculation. Our suggested protocol results in a set of CRC values contributing to the characterization of small animal PET scanners. GATE simulations were also performed to validate the new method and verify the evaluated CRC values. We also demonstrated that the numerical values of this parameter depend on the actual object contrast of the hot region(s) and this mainly comes from the spillover effect. This effect was also studied while analysing the background activity level around the hot rods. We revealed that the calculated background mean values depended on the target contrast in a scanner specific manner. Performing the artificially merged imaging procedure and additional simulations using the micro hollow sphere (MHS) phantom geometry, we also proved that the inactive wall around the hot spheres can have a remarkable impact on the calculated CRC. In conclusion, we have shown that the proposed artificial merging procedure and the commonly used NU4IQ phantom prescribed by the NEMA NU-4 can easily deliver reliable CRC data otherwise unavailable for the NU4IQ phantom in the conventional protocol or the MHS phantom.

Published

2014

7. Development of ⁶⁸Ga-labelled DTPA galactosyl human serum albumin for liver function imaging

Author

Roland, Haubner, David R, Vera, Salman, Farshchi-Heydari, Anna, Helbok, Christine, Rangger, Daniel, Putzer, and Irene J, Virgolini

Subjects

Liver, Albumins, Positron-Emission Tomography, Organometallic Compounds, Animals, Humans, Technetium Tc 99m Pentetate, Gallium Radioisotopes, Tissue Distribution, Pentetic Acid, Radiopharmaceuticals, Technetium Tc 99m Aggregated Albumin, Rats

Abstract

The hepatic asialoglycoprotein receptor is responsible for degradation of desialylated glycoproteins through receptor-mediated endocytosis. It has been shown that imaging of the receptor density using [(99m)Tc]diethylenetriamine pentaacetic acid (DTPA) galactosyl human serum albumin ([(99m)Tc]GSA) allows non-invasive determination of functional hepatocellular mass. Here we present the synthesis and evaluation of [(68)Ga]GSA for the potential use with positron emission tomography (PET).Labelling of GSA with (68)Ga was carried out using a fractionated elution protocol. For quality control thin-layer chromatography (TLC), high-performance liquid chromatography (HPLC) and size exclusion chromatography (SEC) techniques were evaluated. Stability of [(68)Ga]GSA was studied in phosphate-buffered saline (PBS) and human serum. For in vivo evaluation [(68)Ga]GSA distribution in Lewis rats was compared with [(99m)Tc]GSA by using a dual isotope protocol. PET and planar imaging studies were performed using the same scaled molar dose of [(68)Ga]GSA and [(99m)Tc]GSA. Time-activity curves (TAC) for heart and liver were generated and corresponding parameters calculated (t50, t90).[(68)Ga]GSA can be produced with high radiochemical purity. The best TLC methods for determining potential free (68)Ga include 0.1 M sodium citrate as eluent. None of the TLC methods tested were able to determine potential colloids. This can be achieved by SEC. HPLC confirmed high radiochemical purity (98%). Stability after 120 min incubation at 37 °C was high in PBS (95% intact tracer) and low in human serum (∼27% intact tracer). Biodistribution studies simultaneously injecting both tracers showed comparable liver uptake, whereas activity concentration in blood was higher for [(68)Ga]GSA compared to [(99m)Tc]GSA. The [(99m)Tc]GSA TACs exhibited a small degree of hepatic metabolism compared to the [(68)Ga]GSA curves. The mean [(68)Ga]GSA t90 was higher than the mean t90 for [(99m)Tc]GSA. The mean [(68)Ga]GSA t50 was not significantly different from the mean t50 for [(99m)Tc]GSA.This study provides a promising new (68)Ga-labelled compound based on a commercially used kit for imaging the functional hepatocellular mass.

Published

2013

8. Tumor platinum concentration following intraperitoneal administration of cisplatin versus carboplatin in an ovarian cancer model

Author

Danielle D. Jandial, Stephen B. Howell, Minya Pu, Karen Messer, and Salman Farshchi-Heydari

Subjects

Oncology, medicine.medical_specialty, endocrine system diseases, Peritoneal surface, Transplantation, Heterologous, Mice, Nude, Article, Carboplatin, chemistry.chemical_compound, Mice, Internal medicine, Ovarian carcinoma, Cell Line, Tumor, medicine, Animals, Humans, Cystadenocarcinoma, Mice nude, Platinum, Cisplatin, Ovarian Neoplasms, business.industry, Obstetrics and Gynecology, medicine.disease, Cystadenocarcinoma, Serous, Transplantation, chemistry, Cancer research, Female, business, Ovarian cancer, medicine.drug

Abstract

Current intraperitoneal (IP) regimens for the treatment of ovarian cancer rely on cisplatin (DDP) whereas intravenous regimens rely on carboplatin (CBDCA). A major question in the field is whether CBDCA can replace DDP for IP treatment. We compared the uptake of IP administered DDP and CBDCA into human ovarian carcinoma nodules of various sizes growing on the peritoneal surface of nu/nu mice.Human 2008 cells expressing GFP were inoculated IP in nu/nu mice. When small tumor nodules became visible by external imaging, a maximum tolerated dose of DDP, or either an equimolar or equitoxic dose of CBDCA, was injected IP. Platinum (Pt) concentration in tumor nodules was measured by inductively coupled plasma mass spectrometry.A total of 749 tumors harvested from 33 mice were analyzed for Pt concentration. DDP produced a 3.4-fold higher level of Pt in tumor nodules when compared to an equimolar dose of CBDCA (p=0.02). However, when DDP and CBDCA were injected at doses that were equitoxic to the mice, tumor Pt levels were equivalent (p=0.63). Although Pt concentrations of equal-sized nodules were highly variable, tumor Pt content (ng Pt/mg tumor) decreased with increasing nodule size following IP DDP, an effect not seen with IP administration of equitoxic doses of CBDCA (p0.001).These results suggest that IP CBDCA has comparable or better drug penetration when compared to DDP given at equitoxic doses, and thus provide support for replacing DDP with CBDCA in the IP treatment of patients with ovarian cancer.

Published

2009

9. In vivo simultaneous monitoring of two fluorophores with lifetime contrast using a full-field time domain system

Author

Sung-Ho Han, Salman Farshchi-Heydari, Ulas Sunar, and David J. Hall

Subjects

Point spread function, Diagnostic Imaging, Materials science, Time Factors, business.industry, Materials Science (miscellaneous), Mice, Nude, Optical Devices, Fluorescence, Industrial and Manufacturing Engineering, Injections, Light intensity, Mice, Optics, In vivo, Continuous wave, Bioluminescence, Animals, Time domain, Business and International Management, Molecular imaging, business, Fluorescent Dyes

Abstract

Optical molecular imaging of small animals in vivo has witnessed dramatic growth during the past decade. Most commercial systems are based on continuous wave technology and measure solely bioluminescence or fluorescence intensity. Time domain (TD) technology enables the measurement of both intensity and fluorescence lifetime as an additional imaging metric. We have developed a novel, in-house, full-field TD system with dramatically faster acquisition times than available from a commercial TD system. Recent in vivo data from a mouse imaged with the full-field TD system has demonstrated the potential to monitor and discriminate two fluorophores injected simultaneously based on their fluorescence lifetime contrast.

Published

2009

10. Enhanced Delivery of Cisplatin to Intraperitoneal Ovarian Carcinomas Mediated by the Effects of Bortezomib on the Human Copper Transporter 1

Author

Danielle D. Jandial, Gregory I. Elliott, Wolfgang J. Wrasidlo, Stephen B. Howell, Salman Farshchi-Heydari, and Christopher A. Larson

Subjects

Cancer Research, medicine.medical_specialty, Proteasome Endopeptidase Complex, Mice, Nude, Antineoplastic Agents, Biology, Article, Bortezomib, Route of administration, Mice, Drug Delivery Systems, Western blot, hemic and lymphatic diseases, Ovarian carcinoma, Internal medicine, Cell Line, Tumor, medicine, Animals, Humans, Cation Transport Proteins, Peritoneal Neoplasms, Copper Transporter 1, Cisplatin, Ovarian Neoplasms, medicine.diagnostic_test, Cancer, medicine.disease, Boronic Acids, Gene Expression Regulation, Neoplastic, Endocrinology, Cell killing, Oncology, Pyrazines, Cancer research, Proteasome inhibitor, Female, medicine.drug

Abstract

Purpose: The copper transporter 1 (CTR1) is a major influx transporter for platinum drugs. However, the accumulation of cisplatin in human ovarian carcinoma cells is limited by the fact that cisplatin triggers the down-regulation and proteasomal degradation of CTR1, thereby limiting its own uptake. We sought to determine whether proteasome inhibition using bortezomib would prevent human CTR1 (hCTR1) degradation and increase platinum accumulation in ovarian cancer cells. Experimental Design: The effects of bortezomib on human hCTR1 expression and cisplatin accumulation were measured by Western blot, flow cytometric, and confocal digital imaging analyses. Platinum accumulation was measured by inductively coupled plasma mass spectrometry and bortezomib concentrations by liquid chromatography/mass spectrometry. Results: Bortezomib blocked the cisplatin-induced down-regulation of hCTR1 in a concentration-dependent manner and increased cisplatin uptake 1.6- to 2.4-fold. Median effect analysis showed a combination index of 0.37 at 50% cell kill, indicating a high level of synergy. The effect of bortezomib was muted in cells lacking both alleles of CTR1, showing that bortezomib was working primarily through its effect on blocking hCTR1 degradation. I.p. administration of bortezomib produced a peritoneal/plasma area under the curve ratio of 252 in a murine model. I.p. administration of bortezomib before i.p. cisplatin increased platinum accumulation in peritoneal tumors by 33% (P = 0.006). Conclusions: Proteasomal inhibition prevented cisplatin-induced down-regulation of hCTR1 in ovarian cancer cells and enhanced drug uptake and cell killing in a synergistic manner. Bortezomib shows a large pharmacologic advantage when administered i.p. There is a strong rationale for the combined i.p. administration of bortezomib and cisplatin.

Published

2009

11. Analysis of the fluorescence temporal point-spread function in a turbid medium and its application to optical imaging

Author

David J. Hall, Sung-Ho Han, and Salman Farshchi-Heydari

Subjects

Point spread function, Photon, Materials science, Biomedical Engineering, Fluorescence correlation spectroscopy, Models, Biological, Sensitivity and Specificity, Light scattering, Biomaterials, Optics, Nephelometry and Turbidimetry, Optical transfer function, Image Interpretation, Computer-Assisted, Computer Simulation, business.industry, Scattering, Phantoms, Imaging, Reproducibility of Results, Image Enhancement, Fluorescence, Atomic and Molecular Physics, and Optics, Electronic, Optical and Magnetic Materials, Spectrometry, Fluorescence, Microscopy, Fluorescence, Models, Chemical, business, Preclinical imaging, Algorithms

Abstract

A time-domain optical method to evaluate the concentration (n), lifetime (tau), and depth (d) of a fluorescent inclusion is described by the complete analysis of the fluorescence temporal point-spread function (TPSF). The behavior of parameters in the fluorescence TPSF is explored, and we demonstrate the method with experimental data from a localized fluorescent inclusion in scattering media to recover images of n, tau, and d. The method has potential application for in vivo fluorescence imaging.

Published

2009

12. Analytical Method for the Fast Time-Domain Reconstruction of Fluorescent Inclusions In Vitro and In Vivo

Author

David J. Hall, Sung-Ho Han, and Salman Farshchi-Heydari

Subjects

Imagination, Optics and Photonics, Materials science, Time Factors, Light, media_common.quotation_subject, Biophysics, Spectroscopy, Imaging, and Other Techniques, Mice, Nude, Fluorescence, Mice, Optics, In vivo, Image Processing, Computer-Assisted, Animals, Time domain, Exponential decay, media_common, Mice nude, business.industry, Phantoms, Imaging, Models, Chemical, Continuous wave, business, Biological system, Algorithms

Abstract

A novel time-domain optical method to reconstruct the relative concentration, lifetime, and depth of a fluorescent inclusion is described. We establish an analytical method for the estimations of these parameters for a localized fluorescent object directly from the simple evaluations of continuous wave intensity, exponential decay, and temporal position of the maximum of the fluorescence temporal point-spread function. Since the more complex full inversion process is not involved, this method permits a robust and fast processing in exploring the properties of a fluorescent inclusion. This method is confirmed by in vitro and in vivo experiments.

13. Analysis of the fluorescence temporal point-spread function in a turbid medium and its application to optical imaging.

Author

Sung-Ho Han, Salman Farshchi-Heydari, and David J. Hall

Subjects

*HUMAN life cycle, *LIFE cycles (Biology), *DEVELOPMENTAL biology, *HUMAN growth

Abstract

A time-domain optical method to evaluate the concentration (n), lifetime (τ), and depth (d) of a fluorescent inclusion is described by the complete analysis of the fluorescence temporal point-spread function (TPSF). The behavior of parameters in the fluorescence TPSF is explored, and we demonstrate the method with experimental data from a localized fluorescent inclusion in scattering media to recover images of n, τ, and d. The method has potential application for in vivo fluorescence imaging. [ABSTRACT FROM AUTHOR]

Published

2008