Different storage times and their effect on the bending load to failure testing of murine bone tissue

Abstract Cryopreservation is a well-established method for bone storage. However, the ideal timing of mechanical testing after sacrificing the experimental animals is still under discussion and of significant importance to the presentation of accurate results. Therefore, the aim of this study was to investigate and compare different cryopreservation durations to native murine bone and whether there was an influence on mechanical bone testing. For this study the tibias of 57 female C57BL/6 mice—18-weeks of age—were harvested and randomly allocated to one of four groups with varying storage times: (1) frozen at −80 °C for 3 months, (2) frozen at −80 °C for 6 months, (3) frozen at −80 °C for 12 months and (4) native group. The native group was immediately tested after harvesting. The comparison of the mean strength and load to failure rates demonstrated a significant difference between the storage groups compared to the native control (p = 0.007). However, there was no difference in the strength and the load to failure values of bones of all storage groups when compared against each other. Once cryopreservation at −80 °C is performed, no differences of mechanical bone properties are seen up to 12 months of storage. When actual in vivo data is of close interest, immediate testing should be considered and is preferred. If comparison of groups is required and long-time storage is necessary, cryopreservation seems to be an accurate method at present.

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Interference Screw Versus Suture Anchors for Femoral Fixation in Medial Patellofemoral Ligament Reconstruction: A Biomechanical Study

Orthopaedic Journal of Sports Medicine ◽

10.1177/2325967121989282 ◽

2021 ◽

Vol 9 (3) ◽

pp. 232596712198928

Author(s):

Heath P. Gould ◽

Nicholas R. Delaney ◽

Brent G. Parks ◽

Roshan T. Melvani ◽

Richard Y. Hinton

Keyword(s):

Medial Patellofemoral Ligament ◽

Interference Screw ◽

Biomechanical Study ◽

Graft Fixation ◽

Mpfl Reconstruction ◽

Suture Anchors ◽

Femoral Fixation ◽

Significant Difference ◽

Load To Failure ◽

The Mean

Background: Femoral-sided graft fixation in medial patellofemoral ligament (MPFL) reconstruction is commonly performed using an interference screw (IS). However, the IS method is associated with several clinical disadvantages that may be ameliorated by the use of suture anchors (SAs) for femoral fixation. Purpose: To compare the load to failure and stiffness of SAs versus an IS for the femoral fixation of a semitendinosus autograft in MPFL reconstruction. Study Design: Controlled laboratory study. Methods: Based on a priori power analysis, a total of 6 matched pairs of cadaveric knees were included. Specimens in each pair were randomly assigned to receive either SA or IS fixation. After an appropriate reconstruction procedure, the looped end of the MPFL graft was pulled laterally at a rate of 6 mm/s until construct failure. The best-fit slope of the load-displacement curve was then used to calculate the stiffness (N/mm) in a post hoc fashion. A paired t test was used to compare the mean load to failure and the mean stiffness between groups. Results: No significant difference in load to failure was observed between the IS and the SA fixation groups (294.0 ± 61.1 vs 250.0 ± 55.9; P = .352), although the mean stiffness was significantly higher in IS specimens (34.5 ± 9.6 vs 14.7 ± 1.2; P = .004). All IS reconstructions failed by graft pullout from the femoral tunnel, whereas 5 of the 6 SA reconstructions failed by anchor pullout. Conclusion: In this biomechanical study using a cadaveric model of MPFL reconstruction, SA femoral fixation was not significantly different from IS fixation in terms of load to failure. The mean load-to-failure values for both reconstruction techniques were greater than the literature-reported values for the native MPFL. Clinical Relevance: These results suggest that SAs are a biomechanically viable alternative for femoral-sided graft fixation in MPFL reconstruction.

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Surface culture of Steinernema sp. on two solid media and their pathogenicity against Galleria mellonella

Journal of Helminthology ◽

10.1017/s0022149x21000560 ◽

2021 ◽

Vol 95 ◽

Author(s):

C.I. Cortés-Martínez ◽

A.I. Rodríguez-Hernández ◽

M.R. López-Cuellar ◽

N. Chavarría-Hernández

Keyword(s):

Galleria Mellonella ◽

Egg Yolk ◽

Infective Juvenile ◽

Surface Culture ◽

Solid Media ◽

Significant Difference ◽

Bacterial Lawn ◽

The Mean

Abstract The use of native entomopathogenic nematodes as biocontrol agents is a strategy to decrease the environmental impact of insecticides and achieve sustainable agriculture crops. In this study, the effect of the surface culture of Steinernema sp. JAP1 over two solid media at 23–27°C on infective juvenile (IJ) production and pathogenicity against Galleria mellonella larvae were investigated. First, the bacterial lawn on the surface of the media with egg yolk (P2) or chicken liver (Cl) were incubated in darkness at 30°C for 48 and 72 h, and 100 surface-sterilized IJs were added. Four harvests were conducted within the next 35 days and the mean accumulated production was superior on Cl (210 × 103 IJs) than on P2 (135 × 103 IJs), but the productivity decreased up to 10% when the incubation time of the bacterial lawn was of 72 h. The mean pathogenicity of in vitro- and in vivo-produced IJs were of 47–64% and 31%, respectively. It is worth noting that none of the two solid media had a statistically significant difference in IJ pathogenicity. Considering that the maximum multiplication factor of IJs on solid media was 2108 and that the pathogenicity against G. mellonella was outstanding, Steinernema sp. has a good potential for in vitro mass production.

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The Validity of Ultrasound Estimation of Muscle Volumes

Journal of Applied Biomechanics ◽

10.1123/jab.23.3.213 ◽

2007 ◽

Vol 23 (3) ◽

pp. 213-217 ◽

Cited By ~ 18

Author(s):

Benjamin W. Infantolino ◽

Daniel J. Gales ◽

Samantha L. Winter ◽

John H. Challis

Keyword(s):

Vastus Lateralis ◽

Intraclass Correlation ◽

Accurate Method ◽

Muscle Volume ◽

Volume Estimation ◽

Percentage Error ◽

Ultrasound Images ◽

Significant Difference ◽

Hydrostatic Weighing

The purpose of this study was to validate ultrasound muscle volume estimation in vivo. To examine validity, vastus lateralis ultrasound images were collected from cadavers before muscle dissection; after dissection, the volumes were determined by hydrostatic weighing. Seven thighs from cadaver specimens were scanned using a 7.5-MHz ultrasound probe (SSD-1000, Aloka, Japan). The perimeter of the vastus lateralis was identified in the ultrasound images and manually digitized. Volumes were then estimated using the Cavalieri principle, by measuring the image areas of sets of parallel two-dimensional slices through the muscles. The muscles were then dissected from the cadavers, and muscle volume was determined via hydrostatic weighing. There was no statistically significant difference between the ultrasound estimation of muscle volume and that estimated using hydrostatic weighing (p> 0.05). The mean percentage error between the two volume estimates was 0.4% ± 6.9. Three operators all performed four digitizations of all images from one randomly selected muscle; there was no statistical difference between operators or trials and the intraclass correlation was high (>0.8). The results of this study indicate that ultrasound is an accurate method for estimating muscle volumes in vivo.

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Measurement of cation fluxes in rat diaphragm

Proceedings of the Royal Society of London Series B Biological Sciences ◽

10.1098/rspb.1954.0039 ◽

1954 ◽

Vol 142 (909) ◽

pp. 497-513 ◽

Cited By ~ 47

Keyword(s):

Cell Membrane ◽

Ion Concentration ◽

Half Time ◽

Ionic Flux ◽

Simple Diffusion ◽

Apparent Diffusion Coefficients ◽

Significant Difference ◽

Apparent Diffusion ◽

The Mean

Calculation of the ionic flux in isolated mammalian muscle at 38° C required a knowledge of internal ion concentration, the cell dimensions, and the kinetics of exchange across the cell membrane. Muscles soaked in Krebs saline showed no indication of fibre swelling or gain of cell water; there was a small fall of intracellular potassium, accompanied by a large rise of sodium. With proper oxygenation, muscle potassium was constant for several hours; anoxia rapidly produced a fall in potassium and gain of sodium. The use of radioactive tracers showed that potassium was completely exchangeable. The mean half-time for exchange of potassium between tissue and saline was 45 min. Initially the rate was somewhat more rapid, but it finally became steady. There was no significant difference between the rates of entry and exit. Potassium exchange was apparently slowed by diffusion through the interspaces; the calculated exchange rate across the cell membrane had a half-time of 36 min. The mean potassium flux, after correcting for diffusion, was 21 x 10 -12 equiv. cm -2 s -1 . Fibre sodium exchanged with a half-time of about 10 min, and the outward sodium flux was 28 x 10 -12 equiv. cm -2 s -1 . High values were found for the intercellular space, being 26 ml./100 g in soaked diaphragm muscles as measured by inulin. This was confirmed by a method involving radioactive sodium, and the inulin space in vivo was similar. In their passage through the intercellular fluid, inulin, potassium and sodium appear to follow simple diffusion kinetics, and their apparent diffusion coefficients have been estimated.

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Quantitative assessment of choriocapillaris flow deficits in diabetic retinopathy: A swept-source optical coherence tomography angiography study

PLoS ONE ◽

10.1371/journal.pone.0243830 ◽

2020 ◽

Vol 15 (12) ◽

pp. e0243830

Author(s):

Yining Dai ◽

Hao Zhou ◽

Qinqin Zhang ◽

Zhongdi Chu ◽

Lisa C. Olmos de Koo ◽

...

Keyword(s):

Optical Coherence Tomography ◽

Diabetic Retinopathy ◽

Healthy Subjects ◽

Optical Coherence Tomography Angiography ◽

Optical Coherence ◽

Swept Source ◽

Significant Difference ◽

En Face ◽

The Mean

Purpose To quantitatively assess choriocapillaris (CC) flow deficits in eyes with diabetic retinopathy (DR) using swept-source optical coherence tomography angiography (SS-OCTA). Methods Diabetic subjects with different stages of DR and age-matched healthy subjects were recruited and imaged with SS-OCTA. The en face CC blood flow images were generated using previously published and validated algorithms. The percentage of CC flow deficits (FD%) and the mean CC flow deficit size were calculated in a 5-mm-diameter circle centered on the fovea from the 6×6-mm scans. Results Forty-five diabetic subjects and 27 control subjects were included in the study. The CC FD% in diabetic eyes was on average 1.4-fold greater than in control eyes (12.34±4.14% vs 8.82±2.61%, P < 0.001). The mean CC FD size in diabetic eyes was on average 1.4-fold larger than in control eyes (2151.3± 650.8μm2 vs 1574.4±255.0 μm2, P < 0.001). No significant difference in CC FD% or mean CC FD size was observed between eyes with nonproliferative DR and eyes with proliferative DR (P = 1.000 and P = 1.000, respectively). Conclusions CC perfusion in DR can be objectively and quantitatively assessed with FD% and FD size. In the macular region, both CC FD% and CC FD size are increased in eyes with DR. SS-OCTA provides new insights for the investigations of CC perfusion status in diabetes in vivo.

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Factor H (FH) Is Released Slowly and Continuously from Human Endothelial Cells (ECs): FH Is Not Packaged in Weibel-Palade Bodies or Secreted in Response to EC Stimulation

Blood ◽

10.1182/blood.v124.21.4175.4175 ◽

2014 ◽

Vol 124 (21) ◽

pp. 4175-4175

Author(s):

Sarah E Sartain ◽

Nancy A Turner ◽

Hui Shiu-Ki ◽

Charles G. Minard ◽

Joel L Moake

Keyword(s):

Research Funding ◽

Complement Components ◽

Alexa Fluor ◽

Time Points ◽

Significant Difference ◽

The Mean ◽

Von Willebrand ◽

Fund Research

Abstract Introduction Ultra-large von Willebrand factor (ULVWF) strings are synthesized in ECs, packaged in Weibel-Palade Bodies (WPBs), and secreted by stimulated ECs. Complement components studied to date [C3, factor (F) B, FD, FP, FH, FI, C5] are released slowly and continuously from human umbilical vein endothelial cell (HUVEC) cytoplasm and are not packaged in WPBs (PLoS One. 2013;8(3):e59372). In contrast, a recent report (Blood. 2014;123(1):121-5) contended that FH co-localizes with VWF in the WPBs. If this were so, it could have therapeutic importance for the treatment of atypical hemolytic uremic syndrome (aHUS) resulting from deficiency of FH because it might be possible to increase circulating FH levels transiently by administration of the WPB secretagogue, des-amino-D-arginine vasopressin (DDAVP). Hypothesis FH is not co-localized with VWF in WBPs, but rather is released slowly and continuously from EC cytoplasm regardless of cell stimulation. Methods Immunofluorescent Microscopy HUVECs were stimulated with histamine and stained with rabbit anti-VWF plus secondary donkey anti-rabbit Alexa Fluor IgG-488. The cells were then fixed and stained with goat-anti FH plus secondary chicken anti-goat Alexa Fluor IgG-647. The nuclei were detected with DAPI. In vitro VWF and FH from HUVECs HUVECs either were, or were not, stimulated with histamine. Supernatant was collected a variety of times over 7 hrs and assayed for VWF and FH antigen levels by ELISA. VWF assay antibodies (polyclonal): (1) capture, rabbit anti-human VWF (Ramco); (2) detection, goat anti-human VWF (Bethyl) and rabbit anti-goat IgG-HRP (Invitrogen). FH assay antibodies: (1) capture, polyclonal goat anti-human FH (Advanced Research Technologies); (2) detection, monoclonal mouse anti-human FH (Pierce, Thermo Scientific) and polyclonal goat anti-mouse IgG-HRP (Invitrogen). In vivo VWF and FH Plasma samples were obtained from 6 pediatric patients with von Willebrand disease (VWD) being tested for EC release of WPB VWF in response to DDAVP. For each patient, 1 sample was obtained prior to DDAVP administration, and 2 other samples were obtained 1 and 4 hours later. VWF levels were measured in each sample using standard clinical laboratory procedure at an affiliated hospital. FH antigen levels were quantified by ELISA, as above. Results Using non-overlapping spectral secondary detection antibody pairs, VWF was seen in clusters in HUVEC WPBs (Fig. 1A). In contrast, FH was distributed throughout the HUVEC cytoplasm (Fig. 1B). The VWF and FH images did not overlap, indicating that VWF and FH did not co-localize in the WPBs. Fig 1. Immunofluorescent images of HUVECs stained for VWF and FH. Fig 1. Immunofluorescent images of HUVECs stained for VWF and FH. Histamine addition to HUVECs in vitro resulted in ~ 4-fold increases in VWF secreted from HUVEC WPBs at 30 min and 1 hour, and 2-fold increases at 3 hours (Fig 2A). In contrast, FH release was slow and continuous, regardless of histamine stimulation, suggesting that FH is located in EC cytoplasm and is not stored in WPBs (Fig. 2B). Fig 2. In vitro VWF and FH release from ECs under non-stimulated and histamine-stimulated conditions. Fig 2. In vitro VWF and FH release from ECs under non-stimulated and histamine-stimulated conditions. In all 6 patient samples, VWF antigen increased significantly at 1-hour post-DDAVP administration (Fig. 3A). In contrast, FH antigen levels did not change significantly at hour 1 or hour 4, compared to hour 0, indicating that FH is not co-localized and secreted along with VWF from the WPBs of stimulated ECs in vivo (Fig. 3B). Fig 3. (A) Mean responses of VWF antigen to DDAVP, in vivo, with 95% CIs.The mean response was significantly greater 1-hour and 4-hours post-DDAVP compared with baseline (P=0.0085 and 0.0079, respectively). After 1-hour post-DDAVP, the mean response was 201% greater (95% CI: 129%, 314%) than baseline. After 4-hours, the mean response was 174% greater (95% CI: 123%, 247%) than baseline. (B) Responses of FH to DDAVP, in vivo. There was no statistically significant difference in FH response between time points (P=0.77). Fig 3. (A) Mean responses of VWF antigen to DDAVP, in vivo, with 95% CIs.The mean response was significantly greater 1-hour and 4-hours post-DDAVP compared with baseline (P=0.0085 and 0.0079, respectively). After 1-hour post-DDAVP, the mean response was 201% greater (95% CI: 129%, 314%) than baseline. After 4-hours, the mean response was 174% greater (95% CI: 123%, 247%) than baseline. (B) Responses of FH to DDAVP, in vivo. There was no statistically significant difference in FH response between time points (P=0.77). Conclusions We used immunofluorescent microscopy and ELISA assays on samples obtained in vitro and in vivo to demonstrate that FH is not packaged in, or secreted from, the WPBs of stimulated human ECs. FH is, therefore, similar to all other complement components studied to date in that it is released slowly and continuously from ECs and is not influenced by cell stimulation. DDAVP is unlikely to be a viable treatment option for patients with aHUS secondary to deficiency or inhibition of FH. Disclosures Sartain: Hemostasis and Thrombosis Research Society: Research Funding. Turner:Mary R Gibson Foundation: Research Funding; Hinkson Memorial Fund : Research Funding. Moake:Mary R Gibson Foundation: Research Funding; Hinkson Memorial Fund: Research Funding.

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2. Anti-Bacterial Activity Of N-Hexane Extract Of Malacca Leave (Phyllanthus emblica) On Mice (Mus musculus) Inoculated By Staphylococcus epidermidis In Vivo

Jurnal Medika Veterinaria ◽

10.21157/j.med.vet..v15i1.19840 ◽

2021 ◽

Vol 15 (1) ◽

Author(s):

Nada Sarah Syahputri ◽

Nuzul Asmilia ◽

Rinidar Rinidar ◽

Amalia Sutriana ◽

Fakhrurrazi Fakhrurrazi ◽

...

Keyword(s):

Staphylococcus Epidermidis ◽

Positive Control ◽

Negative Control ◽

Hexane Extract ◽

Phyllanthus Emblica ◽

Treatment Groups ◽

Significant Difference ◽

Treatment Data ◽

The Mean

Malacca plant (Phyllanthus emblica) is one of the medicinal plants. The purpose of this study was to determine the effect of n-hexane extract of Malacca (Phyllanthus emblica) leaves on the growth of Staphylococcus epidermidis bacteria in vivo. All mice were first induced by Staphylococcus epidermidis bacteria. Negative control (K1) was given aquadest, positive control (K2) was given ciproflaxacin suspension at doses of 20 mg/kg BW, while K3, K4, and K5 were given n-hexane extract of Malacca leave at dose of 100 mg/kg BW, 200 mg/kg BW, and 300 mg/kg BW. Respectively blood sampling was carried out on the 5th day after treatment. Data were analyzed using one-way analysis of variance (ANOVA). The results showed that the mean (± SD) number of bacterial colonies in K1 was 656x10² cfu/ml. The average number of bacterial colonies in K2 was 2328x10² cfu/ml. The average number of bacterial colonies given n-hexane extract of malacca leave 100 mg/kg BW on K3 was 359,60x10² cfu/ml. The average number of bacterial colonies given n-hexane extract of malacca leave 200 mg/kg BW at K4 was 200x10² cfu/ml and the average number of bacterial colonies given n-hexane extract of malacca leave 300 mg/kg BW at K5 was 3483x10² cfu/ml. The results showed there were no significant difference among treatment groups (P 0.05). N-hexane extract of malacca leave was unable to inhibit the growth of Staphylococcus epidermidis bacteria in vivo

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Assessment of Anthelmintic Resistance of Fasciola spp. against Flunil-L ® and Fasinash®

Bhutan Journal of Natural Resources & Development ◽

10.17102/cnr.2020.51 ◽

2020 ◽

Vol 7 (2) ◽

pp. 43-50

Author(s):

Sonam Dolma ◽

Jigme Tenzin ◽

Jambay Dorjee

Keyword(s):

Confidence Level ◽

Anthelmintic Resistance ◽

Development Of Resistance ◽

Significant Difference ◽

Faecal Egg Count ◽

The Status ◽

Long Time ◽

The Mean ◽

Pre Treatment ◽

Fasciola Spp

Fasciolosis caused by Fasciola spp. is recognized to be one of the major problems affecting health and productivity of cattle in Bhutan. Various anthelmintic drugs are used to treat and control fascioliasis in the country among which, triclabendazole and oxyclozanide are the most common ones. These drugs have been used for a very long time in the country and possibility of development of resistance to these drugs is high. Also, limited studies had been carried out to test their efficacies in the country. Therefore, this study was done to determine the prevalence of fasciolosis in cattle in Maedwang gewog under Thimphu Dzongkhag and assess the status of resistance of Fasciola spp. to Fasinash® and Flunil-L® drugs. A total of 218 faecal samples were collected from cattle and subjected to parasitological test using standard sedimentation technique. The animals positive to Fasciola were treated with Fasinash® (triclabendazole bolus) and Flunil-L® (oxyclozanide+levamisole suspension). The faecal eggs were analyzed 14 days after the treatment by Faecal Egg Count Reduction Test and the efficacy was calculated. The overall prevalence of fasciolosis in the study was 32.11% with a prevalence of 28.80% in Namseling and 36.56% in Khasadrapchu. The mean faecal egg count (epg) of Fasciola spp. detected in Namseling was 0.65 ± 1.53 SD and in Khasadrapchu was 1.03 ± 2.07 SD. There was no significant difference in the mean faecal egg counts in the two chiwogs (p > .05 at 95% confidence level). The overall efficacy of Fasinash® was 86.96% and for Flunil-L ® was 91.38%. Significant difference was observed between pre-treatment and post-treatment in both the treatment groups (p < .05 at 95% confidence level). However, the study implies development of resistance of Fasciola spp. to triclabendazole in the study area.

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Monitoring Gastric Mucosal Carbon Dioxide Pressure Using Gas Tonometry

Anesthesiology ◽

10.1097/00000542-199709000-00008 ◽

1997 ◽

Vol 87 (3) ◽

pp. 504-510 ◽

Cited By ~ 102

Author(s):

Jacques Creteur ◽

Daniel De Backer ◽

Jean-Louis Vincent

Keyword(s):

Carbon Dioxide ◽

Close Correlation ◽

Gastric Tonometry ◽

Time Interval ◽

Equilibration Time ◽

Long Time ◽

Carbon Dioxide Pressure ◽

The Mean

Background Saline gastric tonometry of carbon dioxide has been proposed as a means to assess the adequacy of splanchnic perfusion. However, this technique has several disadvantages, including the long time interval needed for gases to reach equilibrium in saline milieu. Thus the authors evaluated a system that uses a gas-filled instead of a saline-filled gastric balloon. Methods In vitro, we simultaneously placed two tonometry catheters in an equilibration water bath maintained at a predetermined and constant pressure of carbon dioxide (P(CO2)). The first catheter's balloon was filled with air and the second with saline. The performance of gas tonometry was tested by comparing the P(CO2) measurements of the bath obtained via gas tonometry (PgCO2) to the P(CO2) measurements of direct bath samples (PbathCO2). These results were also compared with the P(CO2) measurements obtained simultaneously by saline tonometry (PsCO2). The response time of gas versus saline tonometry was also studied. In vivo, the performance of gas tonometry was tested comparing the measurements of gastric intramucosal P(CO2) obtained by gas tonometry (PgCO2) at different equilibration times with those obtained by saline tonometry (PsCO2) using an equilibration time of 30 min. Two nasogastric tonometry catheters were placed simultaneously in seven stable patients in the intensive care unit. The first balloon was filled with air and the second with saline. Results In vitro, there was a close correlation between PgCO2 and PbathCO2, for each level of PbathCO2, and for each different gas equilibration time. For an equilibration time of 10 min at a PbathCO2 level of approximately 40 mmHg, the bias of the gas device defined as the mean of the differences between PbathCO2 and PgCO2 and its precision defined as the standard deviation of the bias, were -0.3 mmHg and 0.7 mmHg, respectively. Using the same definitions, the bias and precision of saline tonometry were 11.2 mmHg and 1.4 mmHg, respectively. If the equilibration time-dependent correction factor provided by the catheter manufacturer for saline tonometry was applied, the bias and precision were -6.9 mmHg and 2.9 mmHg, respectively. In vivo, using an equilibration time of 10 min for gas and 30 min for saline tonometry, there was a close correlation between the two techniques (r2 = 0.986). A Bland and Altman analysis revealed a bias (+/- 2 SD) of 0.1 +/- 6.8 mmHg. The correlation between the two methods was not improved if we prolonged the equilibration time of the gas tonometer. Conclusions Gas tonometry is comparable to saline tonometry for measuring gastric intramucosal P(CO2). Because gas tonometry is easier to automate, it may offer advantages over saline tonometry.

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P-Glycoprotein Inhibitor Valspodar (PSC 833) Increases the Intracellular Concentrations of Daunorubicin In Vivo in Patients With P-Glycoprotein–Positive Acute Myeloid Leukemia

Journal of Clinical Oncology ◽

10.1200/jco.2000.18.9.1837 ◽

2000 ◽

Vol 18 (9) ◽

pp. 1837-1844 ◽

Cited By ~ 57

Author(s):

U. Tidefelt ◽

J. Liliemark ◽

A. Gruber ◽

E. Liliemark ◽

B. Sundman-Engberg ◽

...

Keyword(s):

Acute Myeloid Leukemia ◽

Myeloid Leukemia ◽

Area Under The Curve ◽

Leukemic Cells ◽

Psc 833 ◽

P Glycoprotein ◽

Significant Difference ◽

The Mean ◽

Acute Myeloid

PURPOSE: The aim of the present study was to evaluate the effect of the cyclosporine derivative valspodar (PSC 833; Amdray, Novartis Pharma, Basel, Switzerland) on the concentration of daunorubicin (dnr) in leukemic blast cells in vivo during treatment.PATIENTS AND METHODS: Ten patients with acute myeloid leukemia (AML) were included. Leukemic cells from seven of the patients were P-glycoprotein (Pgp)–positive. dnr 100 mg/m2was given as a continuous infusion over 72 hours. After 24 hours, a loading dose of valspodar was given, followed by a 36-hour infusion of 10 mg/kg per 24 hours. Blood samples were drawn at regular intervals, and concentrations of dnr and its main metabolite, daunorubicinol, in plasma and isolated leukemic cells were determined by high-pressure liquid chromatography.RESULTS: The mean dnr concentrations in leukemic cells 24 hours after the start of infusion (before valspodar) were 18.8 μmol/L in Pgp-negative samples and 13.5 μmol/L in Pgp-positive samples. After 8 hours of valspodar infusion, these values were 25.8 and 24.0 μmol/L, respectively. The effect of valspodar was evaluated from the ratio of the area under the curve (AUC) for dnr concentration versus time in leukemic cells to the AUC for dnr concentration against time in the plasma. For the seven patients with Pgp-positive leukemia, the mean ratio increased by 52%, from 545 on day 1 to 830 on day 2 (P < .05) when valspodar was given. In the three patients with Pgp-negative leukemia, no significant difference was observed.CONCLUSION: These results strongly suggest that valspodar, by interacting with Pgp, can increase the cellular uptake of dnr in leukemic blasts in vivo.

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