YPD Plus™ (50 ml) ^

使用Lipofectamine™2000转染Stealth™ RNA或者siRNA进入哺乳动物细胞

nM Stealth™ RNA或者siRNA。 2 在30-50％细胞汇合度时进行转染。通常基因阻断的分析至少要在转染后24-72小时进行。低密度转染细胞可以使转染和分析之间更长的间隙更长，从而使由于细胞过度生长造成的细胞活性损害减少到最低。根据靶基因的特性，高密度转染的细胞可能更加适合条件的优化。 3 不要在转染时的培养基中加入抗生素，因为这将会降低细胞转染的效率和导致细胞

蛋白偶联到磁性MagPlex™微球的方法

Monobasic Sodium Phosphate, pH 6.2 by vortex and sonication for approximately 20 seconds. 9.Add 10 μL of 50 mg/mL Sulfo-NHS (diluted in dH2 0) to the microspheres and mix gently by vortex. 10.Add 10 μL of 50 mg/mL EDC (diluted in dH

Mag-Bind Blood RNA Isolation Protocol (for 50ul Blood)

1. Prepare a Lysis Mixture by mixing one volume of Buffer MRB and one volume of isopropanol. For 96 samples, combine15 ml Buffer MRB with 15 ml isopropanol and mix throughly by vortexing. Add 300 ul Lysis Mixture for each sample at step 3. 2. Add 50 ul