Tehryung Kim scite author profile

Methylmercury is an environmental pollutant that biomagnifies in the aquatic food chain with severe consequences for humans and other animals. In an effort to remove this toxin in situ, we have been engineering plants that express the bacterial mercury resistance enzymes organomercurial lyase MerB and mercuric ion reductase MerA. In vivo kinetics experiments suggest that the diffusion of hydrophobic organic mercury to MerB limits the rate of the coupled reaction with MerA (Bizily et al., 2000). To optimize reaction kinetics for organic mercury compounds, themerB gene was engineered to target MerB for accumulation in the endoplasmic reticulum and for secretion to the cell wall. Plants expressing the targeted MerB proteins and cytoplasmic MerA are highly resistant to organic mercury and degrade organic mercury at 10 to 70 times higher specific activity than plants with the cytoplasmically distributed wild-type MerB enzyme. MerB protein in endoplasmic reticulum-targeted plants appears to accumulate in large vesicular structures that can be visualized in immunolabeled plant cells. These results suggest that the toxic effects of organic mercury are focused in microenvironments of the secretory pathway, that these hydrophobic compartments provide more favorable reaction conditions for MerB activity, and that moderate increases in targeted MerB expression will lead to significant gains in detoxification. In summary, to maximize phytoremediation efficiency of hydrophobic pollutants in plants, it may be beneficial to target enzymes to specific subcellular environments.

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Toward detoxifying mercury‐polluted aquatic sediments with rice genetically engineered for mercury resistance

Heaton

Rugh

Kim

et al. 2003

Enviro Toxic and Chemistry

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Mercury contamination of soil and water is a serious problem at many sites in the United States and throughout the world. Plant species expressing the bacterial mercuric reductase gene, merA, convert ionic mercury, Hg(II), from growth substrates to the less toxic metallic mercury, Hg(0). This activity confers mercury resistance to plants and removes mercury from the plant and substrates through volatilization. Our goal is to develop plants that intercept and remove Hg(II) from polluted aquatic systems before it can undergo bacterially mediated methylation to the neurotoxic methylmercury. Therefore, the merA gene under the control of a monocot promoter was introduced into Oryza sativa L. (rice) by particle gun bombardment. This is the first monocot and first wetland-adapted species to express the gene. The merA-expressing rice germinated and grew on semisolid growth medium spiked with sufficient Hg(II) to kill the nonengineered (wild-type) controls. To confirm that the resistance mechanism was the conversion of Hg(II) to Hg(0), seedlings of merA-expressing O. sativa were grown in Hg(II)-spiked liquid medium or water-saturated soil media and were shown to volatilize significantly more Hg(0) than wild-type counterparts. Further genetic manipulation could yield plants with increased efficiency to extract soil Hg(II) and volatilize it as Hg(0) or with the novel ability to directly convert methylmercury to Hg(0).

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Coupling two mercury resistance genes in Eastern cottonwood enhances the processing of organomercury

Lyyra

Meagher

Kim

et al. 2007

Plant Biotechnology Journal

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SummaryEastern cottonwood ( Populus deltoides Bartr. ex Marsh.) trees were engineered to express merA (mercuric ion reductase) and merB (organomercury lyase) transgenes in order to be used for the phytoremediation of mercury-contaminated soils. Earlier studies with Arabidopsis thaliana and Nicotiana tabacum showed that this gene combination resulted in more efficient detoxification of organomercurial compounds than did merB alone, but neither species is optimal for long-term field applications. Leaf discs from in vitro -grown merA, nptII (neomycin phosphotransferase) transgenic cottonwood plantlets were inoculated with Agrobacterium tumefaciens strain C58 carrying the merB and hygromycin resistance ( hptII ) genes. Polymerase chain reaction of shoots regenerated from the leaf discs under selection indicated an overall transformation frequency of 20%. Western blotting of leaves showed that MerA and MerB proteins were produced. In vitro -grown merA / merB plants were highly resistant to phenylmercuric acetate, and detoxified organic mercury compounds two to three times more rapidly than did controls, as shown by mercury volatilization assay. This indicates that these cottonwood trees are reasonable candidates for the remediation of organomercury-contaminated sites.

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Studies on the Effect of Zinc Supply on Growth and Nutrient Uptake in Pecan

Kim

Mills

Wetzstein

2002

Journal of Plant Nutrition

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Zinc (Zn) deficiency is a nutrient disorder observed in pecan (Carya illinoinensis Wangenh. K. Koch) under field conditions, and can cause distorted leaf growth and severe rosetting of shoots. Conducting Zn studies with pecan in the field have been problematic because Zn nutrition is difficult to control. In this study, Zn nutrient disorders were induced in greenhouse-grown pecan seedlings using hydroponic culture. Zinc efficiency was compared in two pecan seedstocks, 'Stuart' and 'Curtis' by evaluating growth response, nutrient uptake, and leaf nutrient analysis. Zinc deficiency symptoms appeared in plants grown in the absence of Zn after six weeks. Deficiency symptoms were characterized by interveinal mottling, followed by interveinal chlorosis, interveinal necrosis, and marginal curling. Symptoms were confined to the youngest most distal three to five leaves. Differences in Zn efficiency between the two seedstock were

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Tehryung Kim

Subcellular Targeting of Methylmercury Lyase Enhances Its Specific Activity for Organic Mercury Detoxification in Plants

Toward detoxifying mercury‐polluted aquatic sediments with rice genetically engineered for mercury resistance

Coupling two mercury resistance genes in Eastern cottonwood enhances the processing of organomercury

Studies on the Effect of Zinc Supply on Growth and Nutrient Uptake in Pecan

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