filter

利用MATLAB语言实现的遗传阈值分割. (using MATLAB genetic threshold segmentation. Using MATLAB genetic threshold Segmentation.)

fbr核 kpcaKPCA的提出者亲自写的程序 (the fbr the nuclear kpcaKPCA the author himself wrote program)

提供一个粒子群算法的实例代码，对于初学者和进一步开发者用很大的帮助(Provide a PSO algorithm code examples for beginners and more developers with great help)

说明：  随机采样，小波基，OMP算法的压缩感知重构matlab代码(Random sampling, wavelet basis, OMP algorithm and reconstruction of matlab code)

说明：  PLD的详细编程开发，主要是针对GAL16V8的的开发(Detailed PLD programming and development, mainly for the development GAL16V8)

Simulink linear pll

matlab函数文件 绘制卫星视角的三维地球视图 清晰逼真(matlab function file rendering three-dimensional perspective of the Earth satellite view vivid)

THIS IS THE MATLAB CODE FOR PTS TO REDUCE PAPR

matlab file for image processing

一个强大的工具分析 寻找 逆转录(逆转录)跟随由聚合酶链反应，该程序定量分析信使核糖核酸。定量表达基因水平，特别是能为低级的丰富信使核糖核酸提供分析工具。(Reverse transcription(RT) followed by PCR is a powerful tool for the detection and quantification of mRNA. It is the most sensitive method for the detection and quantification of gene expression levels, in particular for low abundance mRNA. The relative quantification is based on the expression ratio of a target gene versus a reference gene. Some mathematical models have already been developed to calculate the relative expression ratios, with or without efficiency correction. Normally the PCR efficiency is set at 2 (the max possible value) for the reference and target gene, but a difference in PCR efficiency of 0.03 between the target and reference gene, the falsely calculated difference in expression ratio is 46 in case of Et<Er and 209 in the case of Et>Er. The difference will increase dramatically by higher efficiency differences: i.e. DE=0.05 (27 and 338 ) and DE=0.1 (7.2 and 1083 ) This function computes the efficiency of PCR reaction and is based on my function MYREGR)