該保護劑不含動物蛋白質！，微生物培養液與保護劑混合即可使用。使用該保護劑，細菌的存活率在90 ％以上，遠遠超過使用蔗糖和脫脂牛奶方法的細菌存活率。該試劑無菌過濾處理，包裝是100毫升PET瓶。

使用方法：
1. Simple Culture Preservation:
Add an appropriate volume Lyophilized Buffer to a sterile vial(e.g., 100-500ul). Inoculate the buffer with 10ul of actively growing bacteria. All procedures must be performed aseptically. 
2.Preservation of Large Number of Cells:
Pellet cells from an actively growing culture by centrifugation. Decant the medium and resuspend the cell in an equal volume of Lyophilized Buffer. Transfer the cell solution to a sterile vial.

The freeze drying parameters must be determined for each freeze dryer. However the buffer are 
optimized to freeze drying on the following cycle.
Freezing:30 minutes from ambient to -40℃, hold for 1 hr.
Primary Drying: Increase temperature to -10℃, hold for 16 hours(large volumes 
may require longer reying times).
Secondary Drying:Increase temperature to 20℃, hold for 2 hr.