163 results about "Mercury Bichloride" patented technology

Mercury emissions in an exhaust gas are mitigated. Mercury dichloride is formed upon a surface from a substantial portion of the mercury in the exhaust gas. The mercury dichloride sublimes from the surface, and the sublimed mercury dichloride is subsequently removed from the exhaust stream.

The invention discloses a teapot dates tissue culturing method. The method comprises the steps of clipping teapot dates with a bud stem tip in a large land; cleaning the teapot dates with tap water; putting the teapot dates into alcohol to sterilize; sterilizing by using mercury bichloride; cleaning the teapot dates by using sterile water; inoculating into a starting culture medium; transferring to a meristem culture medium; transferring to a successive transfer culture medium; and finally, finishing the establishment of the whole tissue culture system in a root medium so that the teapot dates tissue is subjected to sterile culture and transplantation under a manually-controlled illumination and temperature condition. In-vitro rapid propagation of the teapot dates is carried out according to the embodiment of the invention, the process from incubation to rooting needs 70 days, the teapot dates tissue can be transplanted to a seedling culture bed on the ground, the induction survival rate is up to 97 percent, the increment reaches 10 times, and the transplantation rooting rate is also up to 95 percent.

The invention discloses a method for improving the embryogenesis efficiency and the plant regeneration efficiency of a stem nodule mustard microspore embryo. The method comprises the following steps of: (1) selecting materials, namely observing flower buds by a microscope, and selecting the flower buds with the diameters of 2-3 mm; (2) performing sterilization, namely performing sterilization by adopting 0.1 percent of mercury bichloride for 12 min, and washing the flower buds by germfree water for three times; (3) extracting pollens, namely adding a B5-13 liquid culture medium for grinding and filtration, and performing centrifugation; (4) performing heat-activation treatment, namely transferring sedimented pollens into an NLN-16 liquid culture medium containing a colchicine solution, culturing the pollens in the dark at the temperature of 32 DEG C for 48-52 hours; (5) performing induction to obtain the embryo, namely performing centrifugation, adding the NLN-13 liquid culture medium, packaging the pollens into a culture dish according to a unit of 1.5 flower buds per culture dish, and culturing the flower buds in the dark at the temperature of 25 DEG C; and (6) performing induction to obtain seedlings, namely after the embryo is formed, transferring the embryo into a B5-3 solid culture medium for culture. The invention creates a novel method of a stem nodule mustard free microspore culture technology and has a wide application prospect in breeding of stem nodule mustards.

The invention relates to an iris germanica Jinwawa tissue culture method. The iris germanica Jinwawa tissue culture method comprises the following steps of 1, selecting a raw material of an iris germanica Jinwawa seedling growing on the land, cutting off young buds with stalks when the young buds are formed between early-March to mid-April, removing outer bracts of the young buds, and flushing by clear water for next use, 2, carrying out immersion disinfection of the cleaned young buds on a superclean workbench orderly by an alcohol solution and a mercury bichloride solution, and flushing by sterile water, 3, removing inner bracts located at lower parts of the young buds, removing top parts and ovaries of the young buds, and introducing the stalks located at insertion parts of the inner bracts into a medium, 4, culturing for a period of time, and when adventitious buds are formed on the insertion parts of the inner bracts, transferring the adventitious buds to a multiplication medium for culture, and 5, culturing for a period of time, cutting off cluster buds formed from the adventitious buds, and culturing the cut cluster buds in a rooting medium to form strong tissue cultured rooting seedlings. The iris germanica Jinwawa tissue culture method has the advantages of simpleness of disinfection, high survival rate and fast breeding speed.