For the isolation of His-tagged proteins under reducing conditions. Immobilized metal ion affinity chromatography (IMAC) still is the most widely used method to obtain high yield of very pure proteins with reasonable effort. ROTI ® Garose His/Ni Beads and ready-to-use columns offer the perfect solution for your specific applications in the field of benchtop column chromatography, for protein isolation in batch processes or under medium pressures (MPLC, FPLC). Depending on the product, our beads are optimally suited for low or high flow rates or when small or large sample volumes are to be purified. Superior recovery rate of pure His-tagged proteins Minimized Nickel leaching Compatible with denaturing and reducing reagents The matrix of ROTI ® Garose-His/Ni NTA products consists of crosslinked and beaded 6 % agarose, NTA-conjugated and charged with divalent Nickel ions. Nickel chelates recognize two histidines that are in close proximity and accessible with good specificity and very high affinity, making the Ni 2+ charged matrix the first choice for all standard applications. The tetradentate NTA crosslinker enables highly efficient binding of His-tagged proteins and leads to high recovery rates with minimized nickel bleeding into the eluate. Directions for use ROTI ® Garose-His/Ni NTA-Beads may be regenerated, making them very cost-effective. The Matrix is stable in all commonly used reagents including denaturing reagents (like 8 M urea, 6 M guanidinium hydrochloride) and (dependent on the respective buffer) reducing substances (for instance ≤30 mM glutathion, ≤10  mM DTT, ≤10 mM DTE, ≤20 mM β-mercaptoethanol und ≤0,3 % SDS). ROTI ® Garose-His/Ni NTA-Beads ROTI ® Garose for biochemistry Nickel charged NTA-agarose beads for affinity chromatography under reducing conditions. 50 % bead suspension in 20 % ethanol. Rapid one-step purification of very pure His-tagged proteins from total lysates High binding capacity for 6xHis-tagged protein Reliably elution and regeneration For batch mode and gravity flow Suitable for The matrix of choice if His-tagged proteins of very small amount shall be isolated from reducing buffer solutions without loss. Directions for use May be autoclaved at 121 °C for 30 mins.