Preparation of a DNA gene probe for detection of mercury resistance genes in gram-negative bacterial communities

Barkay, Tamar; Fouts, David L.; Olson, Betty H.

doi:10.1128/aem.49.3.686-692.1985

Cited by 95 publications

(18 citation statements)

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“…The hypothesis that DNA sequences coding for Hg2+ resistance and volatilization in saline water and freshwater communities had no homology to the characterized mer operon was tested by hybridization of randomly selected representative strains with a mer(Tn2l) DNA probe. Gram-positive strains were excluded from this analysis because their Hg2+ resistance genes bear little homology with mer(Tn21) (30,35) and homology was not sufficient for hybrid formation under the stringency conditions used in this study (8). However, only a minority of the resistant strains were gram positive (ranging from 7.5% in the Vortex Spring community to 1.9% in the coastal marine community).…”

Section: Resultsmentioning

confidence: 99%

“…Aquatic microbial communities adapt to Hg2+ by rapidly volatilizing (and thus eliminating) it from their immediate environment (7). Because Hg2+ reduction to volatile elemental mercury (Hgo) is a well-established resistance mechanism in pure bacterial cultures (35), its role in adaptation and volatilization by the aquatic communities was investigated by DNA-DNA colony hybridization with a DNA probe constructed of a gramnegative mer operon, mer(Tn2J) (8). Although resistance was widely distributed among aerobic .ulturable heterotrophs of adapted communities, DNA sequences homologous to mer were rarely (if at all) detected (7).…”

mentioning

confidence: 99%

“…(iii) Mercuric mercury resistance and volatilization was mediated by bacterial genes that were not homologous to the characterized mer operon. The DNA sequences of mer operons originating in three gram-negative bacteria have been shown to have a high degree of homology (30), and this homology was sufficient to result in cross-hybridization with mer(Tn2l) (8). However, Hg2+-resistant strains that do not hybridize with this probe have been isolated from different environments (2, 10; N. Hamlett, personal communication), and NADPH-dependent mercuric reductase activity has been found in three mer(Tn2l)-negative marine caulobacters (22).…”

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confidence: 99%

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Environmental significance of the potential for mer(Tn21)-mediated reduction of Hg2+ to Hg0 in natural waters

Barkay

Liebert

Gillman

1989

Appl Environ Microbiol

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The role of mer(Tn2l) in the adaptation of aquatic microbial communities to Hg2+ was investigated. Elemental mercury was the sole product of Hg2+ volatilization by freshwater and saline water microbial communities. Bacterial activity was responsible for biotransformation because most microeucaryotes did not survive the exposure conditions, and removal of larger microbes (>1 ,Lm) from adapted communities did not significantly (P > 0.01) reduce Hg2+ volatilization rates. DNA sequences homologous to mer(Tn2l) were found in 50% of Hg2+-resistant bacterial strains representing two freshwater communities, but in only 12% of strains representing two saline communities (the difference was highly significant; P < 0.001). Thus, mer(Tn2l) played a signfficant role in Hg2' resistance among strains isolated from fresh waters, in which microbial activity had a limited role in Hg2+ volatilization. In saline water environments in which microbially mediated volatilization was the major mechanism of Hg2e loss, other bacterial genes coded for this biotransformation.

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Section: Resultsmentioning

confidence: 99%

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confidence: 99%

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confidence: 99%

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Environmental significance of the potential for mer(Tn21)-mediated reduction of Hg2+ to Hg0 in natural waters

Barkay

Liebert

Gillman

1989

Appl Environ Microbiol

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“…This comprehensive approach should pro-Correspondence: K. D. Bruce vide a more representative assessment of the diversity of specific genes in natural bacterial populations. To date, most molecular techniques used for this purpose have involved the direct extraction of DNA (Trevors 1992), followed by DNA cloning (Schmidt et al 1991f, DNA hybridization using specific probes (Barkay et al 1985), polymerase chain readion (PCR) amplification (Britschgi & Giovannoni 1991) or a combination of these approaches.…”

Section: Introductionmentioning

confidence: 99%

Genetic diversity within mer genes directly amplified from communities of noncultivated soil and sediment bacteria

et al. 1995

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Individual merRTAP regions were amplified from DNA directly isolated from soil and sediment samples using consensus primers derived from the Conserved mer sequences of Tn502, Tn22 and pMER419. Soil and sediment samples were taken from four sites in the British Isles; one 'pristine' (SB) and three polluted (SO, SE, T2) with respect to mercury. The sizes of the PCR products amplified (= 1 kb) were consistent with their generation from mer determinants related to the archetypal elements found in Gram negative bacteria. Forty-five individual clones of sequences obtained from these four sites were isolated which hybridized (> 70% homology) to a merRTAP probe from Tn502. The diversity of these amplified mer genes was analysed using Restriction Fragment Length Polymorphism (RFLP) profiling. Fourteen RFLP classes were distinguished, 12 of which proved to be novel and only two of which had been identified in an earlier study of 40 Gram negative mercury resistant bacteria cultured from the same four sites. U P G M A analysis was used to examine the relationships between the 22 dasses of determinant identified. The T2 site, which has the longest history of mercury exposure, was found to have the greatest level of diversity in terms of numbers of classes of determinant, while the SO site, which had the highest mercury levels showed relatively low variation. Variation of mer genes within and between the sequences from cultivated bacteria and from total bacterial DNA shows dearly that analysing only sequences from cultivated organisms results in a gross underestimation of genetic variation.

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“…Первые работы, в которых использовали зонды ДНК для иденти фикации индивидуальных микрорганизмов или группы функциональ но близких микроорганизмов, по-прежнему основывались на необхо димости выделять живой организм на селективных средах и культи вировать его для получения и анализа ДНК [18,19,[21][22][23][24][25][26][27][28]. Серий ные разведения накопительной культуры микроорганизмов или разве дения природных образцов воды либо экстрактов почвы высевали на нитроцеллюлозные фильтры, которые помещали на селективные или неселективные питательные среды.…”

unclassified

Untitled

1994

Biopolym. Cell

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УДК 579.25 Н. А. Козыровская, Г. Л. Ковтунович МОЛЕКУЛЯРНО-БИОЛОГИЧЕСКИЕ МЕТОДЫ ДЕТЕКЦИИ И ИДЕНТИФИКАЦИИ МИКРООРГАНИЗМОВ В ОКРУЖАЮЩЕЙ СРЕДЕ Обзор литературы посвящен новым молекулярным методам детекции и идентификации микроорганизмов в окружающей среде. Обсуждаются преимущества новых методов пе ред традиционно используемыми.Введение. Техногенная деятельность человека постоянно приводит к нарушению взаимоотношений микроорганизмов в окружающей сре де, последствия которого могут оказаться непрогнозируемыми. В свя зи с этим возникает необходимость изучения генетических вариаций в природных микробных сообществах как следствия изменения радиа ционного фона Земли, повышения содержания тяжелых металлов, му тагенных агентов в почве и воде. Однако лишь около 20 % микроор ганизмов, населяющих биосферу, известны науке в настоящее время. Остальные микроорганизмы не выявляются традиционно используе мыми методами. Для исследования изменчивости микроорганизмов под воздействием неблагоприятных факторов окружающей среды нужно, прежде всего, идентифицировать некультивируемые микроор ганизмы и понять их роль в биосфере. Это возможно с использова нием новых молекулярных методов. В прямой зависимости от надеж ных методов диагностики патогенных микроорганизмов находится эпидемиологическая обстановка в обществе. Транспортировка и хра нение пищевых продуктов, вторичное использование сырья, в том чис ле пищевого, сточных вод для ирригации сельскохозяйственных уго дий, орошения спортивных площадок и мытья улиц требуют чувстви тельных и быстрых методов микробиологического контроля за их ка чеством. В медицинской диагностике заболеваний микробной этиоло гии все острее ощущается необходимость разработки простых и до ступных каждой лаборатории методов выявления и идентификации возбудителей болезней. Одной из актуальных в ближайшее время станет проблема мониторинга генетически модифицированных микро организмов (ГММО) в окружающей среде, которые сконструированы для доставки в растение биопестицидов [1], биологического азота [2], защиты растения от действия мороза [3], для биоконтроля бактери альных болезней растения [4] и др. Новые методы для наблюдения за их выживанием, распространением в биоценозе и способностью к генетическому обмену информацией с эндемной микрофлорой долж ны быть высокочувствительными при анализе большого количества проб в короткий срок. Для прогнозирования возможных экологиче ских последствий освобождения ГММО в биосферу важно иметь на дежные методы наблюдения не только за генетически измененными мик роорганизмами, но и их ДНК, освобождающейся после гибели клеток. Будучи защищенной от воздействия эндонуклеаз, она некоторое вре мя сохраняет биологическую активность после смерти клетки и может при благоприятных обстоятельствах вовлекаться в процесс трансфор мации бактерий чаще, чем предполагалось ранее [5].

show abstract

Preparation of a DNA gene probe for detection of mercury resistance genes in gram-negative bacterial communities

Cited by 95 publications

References 50 publications

Environmental significance of the potential for mer(Tn21)-mediated reduction of Hg2+ to Hg0 in natural waters

Environmental significance of the potential for mer(Tn21)-mediated reduction of Hg2+ to Hg0 in natural waters

Genetic diversity within mer genes directly amplified from communities of noncultivated soil and sediment bacteria

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