Clinical and histopathological features of myofibrillar myopathy in Warmblood horses.

BACKGROUND: To report a novel exertional myopathy, myofibrillar myopathy (MFM) in Warmblood (WB) horses. OBJECTIVES: To 1) describe the distinctive clinical and myopathic features of MFM in Warmblood horses and 2) investigate the potential inheritance of MFM in a Warmblood family. STUDY DESIGN: Retrospective selection of MFM cases and prospective evaluation of a Warmblood family. METHODS: Retrospectively, muscle biopsies were selected from Warmblood horses diagnosed with MFM and clinical histories obtained (n = 10). Prospectively, muscle biopsies were obtained from controls (n = 8) and a three generation WB family (n = 11). Samples were assessed for histopathology [scored 0-3], fibre types, cytoskeletal and Z disc protein aggregates, electron microscopic alterations (EM) and muscle glycogen concentrations. RESULTS: Myofibrillar myopathy-affected cases experienced exercise intolerance, reluctance to go forward, stiffness and poorly localised lameness. Abnormal aggregates of the cytoskeletal protein desmin were found in up to 120 type 2a and a few type 2x myofibres of MFM cases. Desmin positive fibres did not stain for developmental myosin, α actinin or dystrophin. Scores for internalised myonuclei (score MFM 0.83 ± 0.67, controls 0.22 ± 0.45), anguloid atrophy (MFM 0.95 ± 0.55, controls 0.31 ± 0.37) and total myopathic scores (MFM 5.85 ± 2.10, controls 1.41 ± 2.17) were significantly higher in MFM cases vs. CONTROLS: Focal Z disc degeneration, myofibrillar disruption and accumulation of irregular granular material was evident in MFM cases. Muscle glycogen concentrations were similar between MFM cases and controls. In the Warmblood family, desmin positive aggregates were found in myofibres of the founding dam and in horses from two subsequent generations. MAIN LIMITATIONS: Restricted sample size due to limited availability of well phenotyped cases. CONCLUSIONS: A distinctive and potentially heritable form of MFM exists in Warmblood horses that present with exercise intolerance and abnormal hindlimb gait. Muscle tissue is characterised by ectopic accumulation of desmin and Z disc and myofibrillar degeneration.

Bioabsorption qualities of chitosan-absorbable vascular templates(1).

PURPOSE:The scope of endovascular surgical techniques has expanded to include the treatment of diseases considered at one time to be amenable only to surgical treatment. The development of the biodegradable template follows as an extension of current permanent stent technology. The goal of our project is to develop and test chitosan as an absorbable template for the vascular system.Ultrapure chitosan, heparin sodium salt and lysozyme, and contrast agents MD-76R and Oxilan-350 were used to give radioopaque quality. Prototype chitosan vascular templates were obtained by a dip coating method in which alternate layers of chitosan were coagulated with nonsolvents or heparin. The amount of loaded and released heparin was determined using Azure II colorimetric assay. In vitro enzymatic degradation of templates was evaluated using lysozyme solutions in phosphate buffered saline. Mechanical properties were analyzed using the Dynamic Mechanical Analyzer, DMA-7 (Perkin Elmer, Foster City, Calif.). The microstructure of freeze-dried templates was investigated by field emission scanning electron microscopy (FE SEM) using an LEO 982 electron microscope (Zeiss, Thornwood, NY).In vivo deployment of the templates was undertaken in 10 full-sized pigs (Sus scrofa). After open expose and control of the iliac artery, a closed balloon catheter technique was used to advance and place the balloon catheter and template. The balloon was then expanded, deploying a Palmaz stent with a chitosan template anchored distally. Patency and deployment of the stent-template complex was confirmed by an arteriogram. The animals were sacrificed at 1, 2, 3, 4, and 5 weeks poststent placement, and arterial sections were taken for microscopic analysis. The amount of chitosan remaining was estimated to determine an in vivo rate of absorption.On hematoxilyn and eosin staining of the section arterial samples, a marked inflammatory response was noted and progressed with duration of in vivo contact. A giant cell foreign body reaction coupled with intense intimal hyperplasia and organized thrombus was also noted and progressed with duration of time in vivo. Also noted was the degradation of the template material with only small remnants of material noted within the giant cell by week 4. Clinically, none of the pigs developed limb ischemia or evidence of thromboembolic events.In this in vivo study, the chitosan template proved to be biodegradable but elicited an intense thrombotic and foreign body reaction despite heparin bonding. Further investigation is ongoing as to decreasing the thrombogenic and antigenic qualities of the template materials by either alteration of the base material or addition of bioactive side chains.

Effects of adenosine and protein kinase C stimulation on mechanical properties of rat cardiac myocytes.

Exposure of the heart to adenosine decreases heart rate and left ventricular developed pressure. However, little is known regarding the influence of adenosine on mechanical properties of isolated ventricular myocytes and the intracellular mechanism(s) by which adenosine acts. Therefore, in the present study we compared the effects of the adenosine receptor agonist R-phenylisopropyladenosine (R-PIA) and protein kinase C (PKC) activator dioctanoylglycerol (DOG) on Ca2+ sensitivity of tension, maximum isometric tension, and velocity of unloaded shortening (Vmax) in enzymatically isolated, drug-treated, and subsequently skinned ventricular myocytes. Neither R-PIA (100 microM) nor DOG (50 microM) affected Ca2+ sensitivity of tension or maximum isometric tension compared with controls. However, both R-PIA and DOG treatment caused approximately 25% decrease in Vmax during maximum activation compared with controls. This suggests adenosine and PKC decrease actin-myosin interaction through an alteration of myofilament proteins. The observed similarity of response after R-PIA and DOG treatment is consistent with the hypothesis that effects of adenosine are mediated by activation of the PKC pathway in isolated ventricular myocytes.