Your search keyword '"Cambra, J. M."' showing total 14 results

1. N-(2-mercaptopropionyl)-glycine enhances in vitro pig embryo production and reduces oxidative stress

Author

Cambra, J. M., Martinez, C. A., Rodriguez-Martinez, H., Martinez, E. A., Cuello, C., and Gil, M. A.

Published

2020

2. The cytokine platelet factor 4 successfully replaces bovine serum albumin for the in vitro culture of porcine embryos

Author

Cambra, J. M., Martinez-Serrano, Cristina, Maside, C., Rodriguez-Martinez, Heriberto, Martinez, E. A., Gil, M. A., Cuello, C., Cambra, J. M., Martinez-Serrano, Cristina, Maside, C., Rodriguez-Martinez, Heriberto, Martinez, E. A., Gil, M. A., and Cuello, C.

Abstract

The cytokine platelet factor 4 (PF4) enhances differentiation and cell viability of different stem cells lines in vitro. This study investigated whether PF4 addition to customary pig embryo semi-defined culture media can improve their developmental outcome (Experiment 1) and ultimately replace the need for bovine serum albumin (BSA, Experiment 2). Experiment 1 added PF4 (100-1000 ng/mL, 0 = control) to NCSU-23 with 0.4 mg/mL BSA culturing 3430 presumptive zygotes. Experiment 2 added PF4 (100 -1000 ng/mL, 0 = Control-PVA) to a BSA-free medium (NCSU-23 with 0.3 mg/mL PVA) culturing 3820 presumptive zygotes. Zygote culture in NCSU-23 with 0.4 mg/mL BSA was used as overall control. All groups of Experiment 1 displayed similar rates of day 2-cleavage (range: 65.0 +/- 10.9 to 70.0 +/- 5.8%); of day 7-blastocyst rates (range: 46.6 +/- 10.0 to 56.4 +/- 8.2%) and of total day 7-blastocyst efficiency (range: 32.3 +/- 8.3 to 37.2 +/- 7.3%). Addition of PF4 did not affect total cell numbers of day 7 blastocysts (range: 44.1 +/- 23.2 to 50.5 +/- 26.4). In Experiment 2, PF4 accelerated embryo development, increasing (P < 0.01) blastocyst yield compared to 0-PF4, and blastocyst formation by day 5 adding PF4 100-500 ng/mL (range: 29.9 +/- 7.8 to 31.8 +/- 5.5%; P < 0.05) compared with BSA-control (17.2 +/- 8.2%) and PF4 1000 ng/mL (15.5 +/- 7.9%); showing similar blastocyst rates (range: 42.0 +/- 11.5 to 49.3 +/- 10.0%), total efficiency (28.0 +/- 8.2 to 32.3 +/- 7.1%) total cell numbers (range: 42.6 +/- 19.3 to 45.7 +/- 23.9) as BSA-controls. In conclusion, although PF4 did not show additive improvement under usual semi-defined, BSA-supplemented embryo media, it successfully replaced BSA sustaining porcine blastocyst production in chemically defined conditions. (C) 2019 Elsevier Inc. All rights reserved., Funding Agencies|Ministry of Science, Innovation and Universities-ERDF, Madrid, Spain [RTI2018-093525-B-I00]; Seneca Foundation, Murcia, SpainFundacion Seneca [19892/GERM/15]; Research Council FORMAS, Stockholm, Sweden [2017e00946]

Published

2020

3. Three-to-5-day weaning-to-estrus intervals do not affect neither efficiency of collection nor in vitro developmental ability of in vivo-derived pig zygotes

Author

Martinez, C. A., Cambra, J. M., Parrilla, I., Lucas, X., Rodriguez-Martinez, Heriberto, Martinez, E. A., Izpisua, J. C., Cuello, C., Gil, M. A., Martinez, C. A., Cambra, J. M., Parrilla, I., Lucas, X., Rodriguez-Martinez, Heriberto, Martinez, E. A., Izpisua, J. C., Cuello, C., and Gil, M. A.

Abstract

An efficient system to collect large numbers of vital zygotes is a pre-requisite for application of zygote genome-editing technology, including development of efficient models for xenotransplantation using pigs. Owing to the sub-optimal in vitro production of zygotes in pigs, efficient collection of in vivo developed zygotes is required. Timing of ovulation is a key factor to sustain efficiency since the interval between pronuclear formation and the first division is very short in pigs. The weaning-to-estrus interval can, due to its inverse relation with length of estrus and time of ovulation, interfere with ovulation and make it asynchronous, which reduces the probability of obtaining zygotes. This retrospective study compared the effects of three weaning-to-estrus intervals of 3, 4 or 5 days on zygote collection efficiency in a total of 17 trials over a 3-year period including 223 sows. Donor sows in groups of 10-15 animals were super-ovulated with eCG 24 h after weaning and those in estrus at 48-72 h post-eCG were immediately treated with hCG, followed by insemination 6 and 24 h thereafter. Collected structures during laparotomy on Day 2 (Day 0: onset of estrus) were morphologically evaluated and only those with a single cell and two visible polar bodies were considered as zygotes. Zygotes were injected with CRISPRCas9 editor mixture and cultured for 6 days to evaluate their developmental ability against non-injected control zygotes. Of all recovered structures (N = 5,468), 67.4%, 30.8% and 1.8% were zygotes, 2-cell embryos and oocytes-degenerated embryos, respectively. The different weaning-to-estrus intervals did not affect either the percentages of collected zygotes (range: 64.1%-70.0%) or the percentages of sows with zygotes at collection time (range: 69.0%-73.3%). The weaning-to-estrus intervals did not affect the in vitro developmental ability of zygotes. After 24 h of culture, 78.1 +/- 2.0% and 95.1 +/- 0.6 (P amp;lt; 0.05) of injected (N = 2,345) and non, Funding Agencies|Seneca Foundation, Murcia, SpainFundacion Seneca [19892/GERM/15]; UCAM (Murcia, Spain) [27094]

Published

2020

4. Porcine blastocyst viability and developmental potential is maintained for 48 h of liquid storage at 25 degrees C without CO2 gassing

Author

Martinez, C. A., Cambra, J. M., Nohalez, A., Parrilla, I., Sanchez-Osorio, J., Roca, J., Rodriguez-Martinez, Heriberto, Gil, M. A., Martinez, E. A., Cuello, C., Martinez, C. A., Cambra, J. M., Nohalez, A., Parrilla, I., Sanchez-Osorio, J., Roca, J., Rodriguez-Martinez, Heriberto, Gil, M. A., Martinez, E. A., and Cuello, C.

Abstract

Short- and medium-term storage of pig embryos has become relevant for commercial application of nonsurgical deep uterine embryo transfer (NsDU-ET) in the light of the strict legal and administrative requirements posed by the International Association for Air Transport (IATA) to allow shipment of liquid nitrogen (LN2) containers and the technical drawbacks when using vitrified embryos. Therefore, this study developed an efficient method for the liquid storage of in vivo-derived porcine blastocysts for a moderate duration (48 h) without controlled CO2 gassing. We evaluated two storage temperatures (25 degrees C and 37 degrees C) and three HEPES-supplemented media: the chemically defined media TL-PVA and NCSU-PVA and the semi-defined medium NCSU-BSA. We observed no differences in survival, hatching rate or final developmental stage between the two temperatures, but storage at 25 degrees C was more efficient to preserve zona pellucida (ZP) integrity. Blastocysts were successfully stored for 24 h in a chemically defined medium. Yet, only 48 h storage in NCSU-BSA medium supported blastocyst development. Although all storage conditions resulted in an embryonic developmental delay, blastocysts stored in NCSU-BSA at either tested temperature could hatch and attain the same final developmental stage as control blastocysts when cultured under standard conditions after storage. Moreover, blastocysts stored at 25 degrees C for 48 h in NCSU-BSA medium could produce pregnancies after surgical transfer. In conclusion, porcine blastocysts maintain their viability and developmental potential after storage in the semi-defined medium NCSU-BSA for at least 48 hat 25 degrees C. (C) 2019 Elsevier Inc. All rights reserved., Funding Agencies|Ministry of Economy and Competitiveness/the European Regional Development Fund [RTC-2016-5448-2, AGL2015-69735-R]; Seneca Foundation, Murcia, Spain [19892/GERM/15]; Research Council FORMAS, Stockholm, Sweden [2017-00946]

Published

2019

5. The revolution in data gathering systems

Author

Cambra, J. M and Trover, W. F

Subjects

Research And Support Facilities (Air)

Abstract

Data acquisition systems used in NASA's wind tunnels from the 1950's through the present time are summarized as a baseline for assessing the impact of minicomputers and microcomputers on data acquisition and data processing. Emphasis is placed on the cyclic evolution in computer technology which transformed the central computer system, and finally the distributed computer system. Other developments discussed include: medium scale integration, large scale integration, combining the functions of data acquisition and control, and micro and minicomputers.

Published

1975

6. Real-time computer data system for the 40- by 80-foot wind tunnel facility at Ames Research Center

Author

Cambra, J. M and Tolari, G. P

Subjects

Research And Support Facilities (Air)

Abstract

The background material and operational concepts of a computer-based system for an operating wind tunnel are described. An on-line real-time computer system was installed in a wind tunnel facility to gather static and dynamic data. The computer system monitored aerodynamic forces and moments of periodic and quasi-periodic functions, and displayed and plotted computed results in real time. The total system is comprised of several off-the-shelf, interconnected subsystems that are linked to a large data processing center. The system includes a central processor unit with 32,000 24-bit words of core memory, a number of standard peripherals, and several special processors; namely, a dynamic analysis subsystem, a 256-channel PCM-data subsystem and ground station, a 60-channel high-speed data acquisition subsystem, a communication link, and static force and pressure subsystems. The role of the test engineer as a vital link in the system is also described.

Published

1975

7. Overvoltage protection network

Author

Cambra, J. M

Subjects

Thermodynamics And Combustion

Abstract

Electrical equipment to be protected from overvoltage is connected with a possible source of overvoltage via an input conductor. A fuse is connected in series with the input conductor. A spark gap is connected between the input conductor and ground for conducting the overvoltage current to ground and for blowing the fuse to open the circuit to the electrical equipment. A pulse attenuator network is provided between the spark gap and the electrical equipment to be protected for attenuating the pulse of energy passing through the fuse and spark gap prior to blowing of the fuse. The pulse attenuator network includes additional shunt spark gaps, series inductance, and a series connection of a twisted shielded pair of conductors having low-voltage insulation.

Published

1974

8. Real time computer data system for the 40 x 80 ft wind tunnel facility at Ames Research Center

Author

Cambra, J. M and Tolari, G. P

Subjects

Computers

Abstract

The wind tunnel realtime computer system is a distributed data gathering system that features a master computer subsystem, a high speed data gathering subsystem, a quick look dynamic analysis and vibration control subsystem, an analog recording back-up subsystem, a pulse code modulation (PCM) on-board subsystem, a communications subsystem, and a transducer excitation and calibration subsystem. The subsystems are married to the master computer through an executive software system and standard hardware and FORTRAN software interfaces. The executive software system has four basic software routines. These are the playback, setup, record, and monitor routines. The standard hardware interfaces along with the software interfaces provide the system with the capability of adapting to new environments.

Published

1974

9. A computer-controlled, on-board data acquisition system for wind-tunnel testing

Author

Finger, H. J and Cambra, J. M

Subjects

Research And Support Facilities (Air)

Abstract

A computer-controlled data acquisition system has been developed for the 40x80-foot wind tunnel at Ames Research Center. The system, consisting of several small onboard units installed in the model and a data-managing, data-displaying ground station, is capable of sampling up to 256 channels of raw data at a total sample rate of 128,000 samples/sec. Complete signal conditioning is contained within the on-board units. The sampling sequence and channel gain selection is completely random and under total control of the ground station. Outputs include a bar-graph display, digital-to-analog converters, and digital interface to the tunnel's central computer, an SEL 840MP. The system can be run stand-alone or under the control of the SEL 840MP.

Published

1974

10. High voltage protection network

Author

Cambra, J. M

Subjects

Electronic Systems

Abstract

Circuit protects technical personnel and test equipment from hazardous currents conducted through safety barriers and into data acquisition equipment. Network isolates energy source, restricts arcing to remote area, and dissipates harmlessly residual energy transient.

Published

1972

11. The cytokine platelet factor 4 successfully replaces bovine serum albumin for the in vitro culture of porcine embryos.

Author

Cambra JM, Martinez CA, Maside C, Rodriguez-Martinez H, Martinez EA, Gil MA, and Cuello C

Subjects

Animals, Dose-Response Relationship, Drug, Fertilization in Vitro veterinary, In Vitro Oocyte Maturation Techniques veterinary, Platelet Factor 4 administration & dosage, Platelet Factor 4 pharmacology, Serum Albumin administration & dosage, Serum Albumin pharmacology, Culture Media chemistry, Embryo Culture Techniques veterinary, Platelet Factor 4 chemistry, Serum Albumin chemistry, Swine embryology

Abstract

The cytokine platelet factor 4 (PF4) enhances differentiation and cell viability of different stem cells lines in vitro. This study investigated whether PF4 addition to customary pig embryo semi-defined culture media can improve their developmental outcome (Experiment 1) and ultimately replace the need for bovine serum albumin (BSA, Experiment 2). Experiment 1 added PF4 (100-1000 ng/mL, 0 = control) to NCSU-23 with 0.4 mg/mL BSA culturing 3430 presumptive zygotes. Experiment 2 added PF4 (100-1000 ng/mL, 0 = Control-PVA) to a BSA-free medium (NCSU-23 with 0.3 mg/mL PVA) culturing 3820 presumptive zygotes. Zygote culture in NCSU-23 with 0.4 mg/mL BSA was used as overall control. All groups of Experiment 1 displayed similar rates of day 2-cleavage (range: 65.0 ± 10.9 to 70.0 ± 5.8%); of day 7-blastocyst rates (range: 46.6 ± 10.0 to 56.4 ± 8.2%) and of total day 7-blastocyst efficiency (range: 32.3 ± 8.3 to 37.2 ± 7.3%). Addition of PF4 did not affect total cell numbers of day 7 blastocysts (range: 44.1 ± 23.2 to 50.5 ± 26.4). In Experiment 2, PF4 accelerated embryo development, increasing (P < 0.01) blastocyst yield compared to 0-PF4, and blastocyst formation by day 5 adding PF4 100-500 ng/mL (range: 29.9 ± 7.8 to 31.8 ± 5.5%; P < 0.05) compared with BSA-control (17.2 ± 8.2%) and PF4 1000 ng/mL (15.5 ± 7.9%); showing similar blastocyst rates (range: 42.0 ± 11.5 to 49.3 ± 10.0%), total efficiency (28.0 ± 8.2 to 32.3 ± 7.1%) total cell numbers (range: 42.6 ± 19.3 to 45.7 ± 23.9) as BSA-controls. In conclusion, although PF4 did not show additive improvement under usual semi-defined, BSA-supplemented embryo media, it successfully replaced BSA sustaining porcine blastocyst production in chemically defined conditions., Competing Interests: Declaration of competing interest None of the authors have any conflicts of interest to declare., (Copyright © 2019 Elsevier Inc. All rights reserved.)

Published

2020

12. Three-to-5-day weaning-to-estrus intervals do not affect neither efficiency of collection nor in vitro developmental ability of in vivo-derived pig zygotes.

Author

Martinez CA, Cambra JM, Parrilla I, Lucas X, Rodriguez-Martinez H, Martinez EA, Izpisua JC, Cuello C, and Gil MA

Subjects

Animals, Embryo Culture Techniques veterinary, Embryo, Mammalian, Insemination, Artificial veterinary, Retrospective Studies, Superovulation drug effects, Swine embryology, Time Factors, Tissue and Organ Harvesting, Chorionic Gonadotropin pharmacology, Oocytes, Swine physiology

Abstract

An efficient system to collect large numbers of vital zygotes is a pre-requisite for application of zygote genome-editing technology, including development of efficient models for xenotransplantation using pigs. Owing to the sub-optimal in vitro production of zygotes in pigs, efficient collection of in vivo developed zygotes is required. Timing of ovulation is a key factor to sustain efficiency since the interval between pronuclear formation and the first division is very short in pigs. The weaning-to-estrus interval can, due to its inverse relation with length of estrus and time of ovulation, interfere with ovulation and make it asynchronous, which reduces the probability of obtaining zygotes. This retrospective study compared the effects of three weaning-to-estrus intervals of 3, 4 or 5 days on zygote collection efficiency in a total of 17 trials over a 3-year period including 223 sows. Donor sows in groups of 10-15 animals were super-ovulated with eCG 24 h after weaning and those in estrus at 48-72 h post-eCG were immediately treated with hCG, followed by insemination 6 and 24 h thereafter. Collected structures during laparotomy on Day 2 (Day 0: onset of estrus) were morphologically evaluated and only those with a single cell and two visible polar bodies were considered as zygotes. Zygotes were injected with CRISPR-Cas9 editor mixture and cultured for 6 days to evaluate their developmental ability against non-injected control zygotes. Of all recovered structures (N = 5,468), 67.4%, 30.8% and 1.8% were zygotes, 2-cell embryos and oocytes-degenerated embryos, respectively. The different weaning-to-estrus intervals did not affect either the percentages of collected zygotes (range: 64.1%-70.0%) or the percentages of sows with zygotes at collection time (range: 69.0%-73.3%). The weaning-to-estrus intervals did not affect the in vitro developmental ability of zygotes. After 24 h of culture, 78.1 ± 2.0% and 95.1 ± 0.6 (P < 0.05) of injected (N = 2,345) and non-injected (N = 335) zygotes, respectively, developed to 2-to-4-cell embryo stage. The total efficiency of the system was 64.1 ± 2.2% and 85.8 ± 1.5% (P < 0.05) for injected and non-injected zygotes, respectively. In conclusion, the results indicate that neither the efficiency of collecting in vivo derived porcine zygotes from superovulated sows nor the zygote ability to develop to blastocyst after cytoplasmic genome-editing injection were affected by a weaning-to-estrus interval between 3-to-5 days., (Copyright © 2019 Elsevier Inc. All rights reserved.)

Published

2020

13. Porcine blastocyst viability and developmental potential is maintained for 48 h of liquid storage at 25 °C without CO 2 gassing.

Author

Martinez CA, Cambra JM, Nohalez A, Parrilla I, Sanchez-Osorio J, Roca J, Rodriguez-Martinez H, Gil MA, Martinez EA, and Cuello C

Subjects

Animals, Embryo Transfer methods, Embryo Transfer veterinary, Embryo, Mammalian, Embryonic Development, Female, Pregnancy, Time Factors, Blastocyst physiology, Embryo Culture Techniques veterinary, Swine embryology

Abstract

Short- and medium-term storage of pig embryos has become relevant for commercial application of non-surgical deep uterine embryo transfer (NsDU-ET) in the light of the strict legal and administrative requirements posed by the International Association for Air Transport (IATA) to allow shipment of liquid nitrogen (LN 2 ) containers and the technical drawbacks when using vitrified embryos. Therefore, this study developed an efficient method for the liquid storage of in vivo-derived porcine blastocysts for a moderate duration (48 h) without controlled CO 2 gassing. We evaluated two storage temperatures (25 °C and 37 °C) and three HEPES-supplemented media: the chemically defined media TL-PVA and NCSU-PVA and the semi-defined medium NCSU-BSA. We observed no differences in survival, hatching rate or final developmental stage between the two temperatures, but storage at 25 °C was more efficient to preserve zona pellucida (ZP) integrity. Blastocysts were successfully stored for 24 h in a chemically defined medium. Yet, only 48 h storage in NCSU-BSA medium supported blastocyst development. Although all storage conditions resulted in an embryonic developmental delay, blastocysts stored in NCSU-BSA at either tested temperature could hatch and attain the same final developmental stage as control blastocysts when cultured under standard conditions after storage. Moreover, blastocysts stored at 25 °C for 48 h in NCSU-BSA medium could produce pregnancies after surgical transfer. In conclusion, porcine blastocysts maintain their viability and developmental potential after storage in the semi-defined medium NCSU-BSA for at least 48 h at 25 °C., (Copyright © 2019 Elsevier Inc. All rights reserved.)

Published

2019

14. High pre-freezing sperm dilution improves monospermy without affecting the penetration rate in porcine IVF.

Author

Martinez CA, Cambra JM, Maside C, Cuello C, Roca J, Martinez EA, Parrilla I, and Gil MA

Subjects

Acrosome ultrastructure, Animals, Embryo Culture Techniques veterinary, Embryonic Development, Fertilization, Fertilization in Vitro methods, Male, Semen Analysis veterinary, Semen Preservation methods, Fertilization in Vitro veterinary, Semen Preservation veterinary, Swine

Abstract

The high incidence of polyspermy is still an unresolved problem for the production of in vitro-produced porcine embryos. In this work, we modified the usual sperm processing sequence for in vitro fertilization (IVF), and the spermatozoa from four boars were frozen directly at a low sperm concentration of 20 × 10 6 sperm/mL (high pre-freezing sperm dilution group; F20), thawed and processed for IVF in three replicates. Spermatozoa from the same boars frozen at a conventional concentration (1000 × 10 6 sperm/mL) were used as the control group. The post-thaw sperm quality evaluation demonstrated that despite there being no differences in the percentage of motile spermatozoa between groups, the proportion of live spermatozoa with intact acrosomes was significantly higher in the F20 group than in the control. The in vitro penetration rate was also similar between groups; however, the co-incubation of oocytes with F20 sperm increased monospermy, IVF efficiency, cleavage rate and the efficiency of blastocyst formation compared with the results for oocytes co-incubated with control spermatozoa. These results indicate, for the first time, that a high pre-freezing sperm dilution increases monospermy without affecting penetration rates, thereby increasing blastocyst formation., (Copyright © 2019 Elsevier Inc. All rights reserved.)

Published

2019