3 research outputs found
Modification of Round Robin and Best CQI Scheduling Method for 3GPP LTE Downlink
In the case of downlink LTE, scheduler is an important element which
assigns RB allocation for different users in a cell. RB is the smallest element
which can be assigned by scheduler. This work proposes a new scheduler
algorithm by considering the tradeoff balance between throughput and fairness
among users. The proposed scheduler combines the benefit from the Best CQI and Round Robin Scheduler. The first time slot applies a Round Robin algorithm in the basis of a continuity
in user sequence at the entire sub frames. The second time slot applies the Best CQI algorithm with a fairness
enhancement. At 15dB SNR, the throughput of each scheduler is 61.2Mbps for Best CQI scheduler, 32.3Mbps for Round Robin scheduler, and 48Mbps for
the proposed scheduler. Based on Jain’s Fairness Index, the proposed scheduler
has a fairness index of 0.97. For 20 users at 5MHz bandwidth, the average
queuing delay gives the value of 5ms for Round
Robin scheduler, 29.38ms for Best CQI
scheduler, and 0.94ms for the proposed scheduler
PERUBAHAN VIABILITAS DAN STRUKTUR SUBSELULER SPERMATOZOA DOMBA SETELAH PENGERINGBEKUAN
Several methods i.e. cooling, freezing, and freeze-drying have been widely used to preserve spermatozoa with various degree of success. Freeze-drying appears to provide a method to preserve spermatozoa in a dry state without requiring liquid nitrogen for storing frozen spermatozoa. Freeze-drying procedures can have a detrimental effect on plasma membrane and acrosomal cap of the spermatozoa. In this experiment study, the viability and subcellular changes of freeze-dried ram spermatozoa were evaluated using staining method and scanning electron microscopy. The results revealed that all freeze-dried spermatozoa were dead following evaluation using eosin staining and Hoechst-propidium iodide staining methods. Morover, plasma membrane and acrosomal cap of freeze-dried ram spermatozoa was disrupted observed using scanning electron microscope.</em
PERUBAHAN VIABILITAS DAN STRUKTUR SUBSELULER SPERMATOZOA DOMBA SETELAH PENGERINGBEKUAN
Several methods i.e. cooling, freezing, and freeze-drying have been widely used to preserve spermatozoa with various degree of success. Freeze-drying appears to provide a method to preserve spermatozoa in a dry state without requiring liquid nitrogen for storing frozen spermatozoa. Freeze-drying procedures can have a detrimental effect on plasma membrane and acrosomal cap of the spermatozoa. In this experiment study, the viability and subcellular changes of freeze-dried ram spermatozoa were evaluated using staining method and scanning electron microscopy. The results revealed that all freeze-dried spermatozoa were dead following evaluation using eosin staining and Hoechst-propidium iodide staining methods. Morover, plasma membrane and acrosomal cap of freeze-dried ram spermatozoa was disrupted observed using scanning electron microscope.</div