Your search keyword '"EST database"' showing total 96 results

1. The architecture of pre-mRNAs affects mechanisms of splice-site pairing

Author

Fox-Walsh, KL, Dou, YM, Lam, BJ, Hung, SP, Baldi, PF, and Hertel, KJ

Subjects

alternative splicing, bioinformatics, EST database, intron length

Published

2005

2. Development of a panel of unigene-derived polymorphic EST–SSR markers in lentil using public database information

Author

Debjyoti Sen Gupta, Peng Cheng, Gaurav Sablok, Dil Thavarajah, Pushparajah Thavarajah, Clarice J. Coyne, Shiv Kumar, Michael Baum, and Rebecca J. McGee

Subjects

Lens culinaris, EST–SSRs, Functional annotation, Unigene sequences, EST database, Genetic resources, Agriculture, Agriculture (General), S1-972

Abstract

Lentil (Lens culinaris Medik.), a diploid (2n = 14) with a genome size greater than 4000 Mbp, is an important cool season food legume grown worldwide. The availability of genomic resources is limited in this crop species. The objective of this study was to develop polymorphic markers in lentil using publicly available curated expressed sequence tag information (ESTs). In this study, 9513 ESTs were downloaded from the National Center for Biotechnology Information (NCBI) database to develop unigene-based simple sequence repeat (SSR) markers. The ESTs were assembled into 4053 unigenes and then analyzed to identify 374 SSRs using the MISA microsatellite identification tool. Among the 374 SSRs, 26 compound SSRs were observed. Primer pairs for these SSRs were designed using Primer3 version 1.14. To classify the functional annotation of ESTs and EST–SSRs, BLASTx searches (using E-value 1 × 10−5) against the public UniProt (http://www.uniprot.org/) and NCBI (http://www.ncbi.nlh.nih.gov/) databases were performed. Further functional annotation was performed using PLAZA (version 3.0) comparative genomics and GO annotation was summarized using the Plant GO slim category. Among the synthesized 312 primers, 219 successfully amplified Lens DNA. A diverse panel of 24 Lens genotypes was used to identify polymorphic markers. A polymorphic set of 57 markers successfully discriminated the test genotypes. This set of polymorphic markers with functional annotation data could be used as molecular tools in lentil breeding.

Published

2016

3. Transcriptome Analysis in the Saccharinae

Author

Nishiyama, Milton Yutaka, Jr, Vicente, Fabio, Sato, Paloma Mieko, Ferreira, Savio Siqueira, Feltus, Frank Alex, Souza, Glaucia Mendes, and Paterson, Andrew H., editor

Published

2013

4. Maternal Genetic Information Stored in Fertilized Eggs of the Ascidian, Halocynthia roretzi

Author

Makabe, Kazuhiro W., Kawashima, Takeshi, Kawashima, Shuichi, Sasakura, Yasunori, Ishikawa, Hisayoshi, Kawamura, Hiroshi, Kanehisa, Minoru, Nishikata, Takahito, Nishida, Hiroki, Sawada, Hitoshi, editor, Yokosawa, Hideyoshi, editor, and Lambert, Charles C., editor

Published

2001

5. Development and Validation of Single Nucleotide Polymorphisms (SNPs) Markers from Two Transcriptome 454-Runs of Turbot (Scophthalmus maximus) Using High-Throughput Genotyping

Author

Roman Vilas, Paulino Martinez, Carmen Bouza, Carlos Fernandez, Jose-Antonio Alvarez-Dios, and Manuel Vera

Subjects

turbot, Scophthalmus maximus, SNP validation, EST database, non-synonymous substitution, high-throughput genotyping, Biology (General), QH301-705.5, Chemistry, QD1-999

Abstract

The turbot (Scophthalmus maximus) is a commercially valuable flatfish and one of the most promising aquaculture species in Europe. Two transcriptome 454-pyrosequencing runs were used in order to detect Single Nucleotide Polymorphisms (SNPs) in genes related to immune response and gonad differentiation. A total of 866 true SNPs were detected in 140 different contigs representing 262,093 bp as a whole. Only one true SNP was analyzed in each contig. One hundred and thirteen SNPs out of the 140 analyzed were feasible (genotyped), while Ш were polymorphic in a wild population. Transition/transversion ratio (1.354) was similar to that observed in other fish studies. Unbiased gene diversity (He) estimates ranged from 0.060 to 0.510 (mean = 0.351), minimum allele frequency (MAF) from 0.030 to 0.500 (mean = 0.259) and all loci were in Hardy-Weinberg equilibrium after Bonferroni correction. A large number of SNPs (49) were located in the coding region, 33 representing synonymous and 16 non-synonymous changes. Most SNP-containing genes were related to immune response and gonad differentiation processes, and could be candidates for functional changes leading to phenotypic changes. These markers will be useful for population screening to look for adaptive variation in wild and domestic turbot.

Published

2013

6. Lachesana tarabaevi, an expert in membrane-active toxins.

Author

Kuzmenkov, Alexey I., Sachkova, Maria Y., Kovalchuk, Sergey I., Grishin, Eugene V., and Vassilevski, Alexander A.

Subjects

*SPIDER venom, *PEPTIDE antibiotics, *EXPRESSED sequence tag (Genetics), *POLYPEPTIDES, *TOXICITY testing

Abstract

In the present study, we show that venom of the ant spider Lachesana tarabaevi is unique in terms of molecular composition and toxicity. Whereas venom of most spiders studied is rich in disulfide-containing neurotoxic peptides, L. tarabaevi relies on the production of linear (no disulfide bridges) cytolytic polypeptides. We performed full-scale peptidomic examination of L. tarabaevi venom supported by cDNA library analysis. As a result, we identified several dozen components, and a majority (~80% of total venom protein) exhibited membrane-active properties. In total, 33 membrane-interacting polypeptides (length of 18-79 amino acid residues) comprise five major groups: repetitive polypeptide elements (Rpe), latarcins (Ltc), met-lysines (MLys), cyto-insectotoxins (CIT) and latartoxins (LtTx). Rpe are short (18 residues) amphiphilic molecules that are encoded by the same genes as antimicrobial peptides Ltc 4a and 4b. Isolation of Rpe confirms the validity of the iPQM (inverted processing quadruplet motif) proposed to mark the cleavage sites in spider toxin precursors that are processed into several mature chains. MLys (51 residues) present 'idealized' amphiphilicity when modelled in a helical wheel projection with sharply demarcated sectors of hydrophobic, cationic and anionic residues. Four families of CIT (61-79 residues) are the primary weapon of the spider, accounting for its venom toxicity. Toxins from the CIT 1 and 2 families have a modular structure consisting of two shorter Ltc-like peptides. We demonstrate that in CIT 1a, these two parts act in synergy when they are covalently linked. This finding supports the assumption that CIT have evolved through the joining of two shorter membrane-active peptides into one larger molecule. [ABSTRACT FROM AUTHOR]

Published

2016

7. terMITEs: miniature inverted-repeat transposable elements (MITEs) in the termite genome (Blattodea: Termitoidae).

Author

Luchetti, Andrea

Subjects

*TERMITES, *TRANSPOSONS, *TANDEM repeats, *GENETIC databases, *DNA copy number variations, *NUCLEOTIDE sequencing

Abstract

Transposable elements (TEs) are discrete DNA sequences which are able to replicate and jump into different genomic locations. Miniature inverted-repeats TEs (MITEs) are non-autonomous DNA elements whose origin is still poorly understood. Recently, some MITEs were found to contain core repeats that can be arranged in tandem arrays; in some instances, these arrays have even given rise to satellite DNAs in the (peri)centromeric region of the host chromosomes. I report the discovery and analysis of three new MITEs found in the genome of several termite species (hence the name terMITEs) in two different families. For two of the MITEs ( terMITE1- Tc1/mariner superfamily; terMITE2- piggyBac superfamily), evidence of past mobility was retrieved. Moreover, these two MITEs contained core repeats, 16 bp and 114 bp long respectively, exhibiting copy number variation. In terMITE2, the tandem duplication appeared associated with element degeneration, in line with a recently proposed evolutionary model on MITEs and the origin of tandem arrays. Concerning their genomic distribution, terMITE1 and terMITE3 appeared more frequently inserted close to coding regions while terMITE2 was mostly associated with TEs. Although MITEs are commonly distributed in coding regions, terMITE2 distribution is in line with that of other insects' piggyBac-related elements and of other small TEs found in termite genomes. This has been explained through insertional preference rather than through selective processes. Data presented here add to the knowledge on the poorly exploited polyneopteran genomes and will provide an interesting framework in which to study TEs' evolution and host's life history traits. [ABSTRACT FROM AUTHOR]

Published

2015

8. 斑茅过氧化氢酶基因(EaCAT-la) 克隆与序列分析.

Author

刘洋, 姚艳丽, 胡小文, 徐磊, 邢淑莲, and 张树珍

Abstract

Eriantkus arundinaceus ( Retz. ) Jesw. is one of the most important species of sugarcane related species, and with strong resistance. In this paper, one novel full-length catalase gene(EaCAT-l a, GenBank Accession number KF864223) DNA sequence was cloned by blasting the Sacckarum L. EST database using sorghum CAT gene (GenBank Accession number XM 002437586. 1) cDNA sequence as a querying probe. EaCAT-la was 3831 bp, containing 8 exons and 7 introns, length of cDNA was 1532 bp, containing 10 bp of 5 'untranslated region( UTR) and 43 bp of the 3'UTR, and a 1479 bp open reading frame encoding a 492 amino acid sequence of the protein which has a conserved domain of catalase belonging CAT family. The putative EaCAT-la protein sequence was very homologous with sorghum, rice, maize and other species, and have shown a high conservatism by homologous evolutionary analysis. [ABSTRACT FROM AUTHOR]

Published

2015

9. Physiological and proteomic analyses of salt stress response in the halophyte H alogeton glomeratus.

Author

WANG, JUNCHENG, MENG, YAXIONG, LI, BAOCHUN, MA, XIAOLE, LAI, YONG, SI, ERJING, YANG, KE, XU, XIANLIANG, SHANG, XUNWU, WANG, HUAJUN, and WANG, DI

Subjects

*EFFECT of salt on plants, *PLANT proteomics, *PROTEOMICS, *HALOPHYTES, *HALOGETON glomeratus, *LIVESTOCK poisoning plants, *CHENOPODIACEAE

Abstract

Very little is known about the adaptation mechanism of Chenopodiaceae H alogeton glomeratus, a succulent annual halophyte, under saline conditions. In this study, we investigated the morphological and physiological adaptation mechanisms of seedlings exposed to different concentrations of NaCl treatment for 21 d. Our results revealed that H . glomeratus has a robust ability to tolerate salt; its optimal growth occurs under approximately 100 m m NaCl conditions. Salt crystals were deposited in water-storage tissue under saline conditions. We speculate that osmotic adjustment may be the primary mechanism of salt tolerance in H . glomeratus, which transports toxic ions such as sodium into specific salt-storage cells and compartmentalizes them in large vacuoles to maintain the water content of tissues and the succulence of the leaves. To investigate the molecular response mechanisms to salt stress in H . glomeratus, we conducted a comparative proteomic analysis of seedling leaves that had been exposed to 200 m m NaCl for 24 h, 72 h and 7 d. Forty-nine protein spots, exhibiting significant changes in abundance after stress, were identified using matrix-assisted laser desorption ionization tandem time-of-flight mass spectrometry ( MALDI- TOF/ TOF MS/ MS) and similarity searches across EST database of H . glomeratus. These stress-responsive proteins were categorized into nine functional groups, such as photosynthesis, carbohydrate and energy metabolism, and stress and defence response. [ABSTRACT FROM AUTHOR]

Published

2015

10. Trichoplaxin — A new membrane-active antimicrobial peptide from placozoan cDNA.

Author

Simunić, Juraj, Petrov, Dražen, Bouceba, Tahar, Kamech, Nédia, Benincasa, Monica, and Juretić, Davor

Subjects

*ANTI-infective agents, *ANTISENSE DNA, *PLACOZOA, *SIGNAL peptides, *AMINO acid sequence, *GRAM-positive bacteria

Abstract

Abstract: A method based on the use of signal peptide sequences from antimicrobial peptide (AMP) precursors was used to mine a placozoa expressed sequence tag database and identified a potential antimicrobial peptide from Trichoplax adhaerens. This peptide, with predicted sequence FFGRLKSVWSAVKHGWKAAKSR is the first AMP from a placozoan species, and was named trichoplaxin. It was chemically synthesized and its structural properties, biological activities and membrane selectivity were investigated. It adopts an α-helical structure in contact with membrane-like environments and is active against both Gram-negative and Gram-positive bacterial species (including MRSA), as well as yeasts from the Candida genus. The cytotoxic activity, as assessed by the haemolytic activity against rat erythrocytes, U937 cell permeabilization to propidium iodide and MCF7 cell mitochondrial activity, is significantly lower than the antimicrobial activity. In tests with membrane models, trichoplaxin shows high affinity for anionic prokaryote-like membranes with good fit in kinetic studies. Conversely, there is a low affinity for neutral eukaryote-like membranes and absence of a dose dependent response. With high selectivity for bacterial cells and no homologous sequence in the UniProt, trichoplaxin is a new potential lead compound for development of broad-spectrum antibacterial drugs. [Copyright &y& Elsevier]

Published

2014

11. Development, inheritance and evaluation of 55 novel single nucleotide polymorphism markers for parentage assignment in the Pacific oyster ( Crassostrea gigas).

Author

Jin, Yu-Lin, Kong, Ling-Feng, Yu, Hong, and Li, Qi

Abstract

Expressed sequence tags (ESTs) are essential to ascertain gene function, but also to identify polymorphic gene-associated single nucleotide polymorphisms (SNPs) (type I markers) suitable for map construction and population analysis in the Pacific oyster ( Crassostrea gigas). In this study, a total of 48,769 putative SNPs were detected from 46,171 ESTs of the Pacific oyster. Fifty-five gene-derived SNPs were isolated and characterized by means of high resolution melting analysis. The observed and expected heterozygosities ranged from 0.063-0.563 and 0.091-0.448, with an average of 0.284 and 0.279, respectively. The SNPs were tested on 6 families of C. gigas for examination of inheritance mode of SNPs. One hundred and thirty-two tests of segregation ratios at 48 loci revealed 30 (22 %) significant departures from expected Mendelian ratios, but no null allele was detected. The power of these SNPs in parentage assignment was evaluated, and the real data demonstrated that 17 % of all real offspring were unambiguously assigned parents with 30 SNPs, and 100 % of the offspring were correctly allocated to their parents when 40 or more SNPs were used. The results obtained in this study suggest that gene-derived SNPs will complement the currently available microsatellite markers and may be useful for comparative mapping, marker-assisted selection and evolutionary studies. [ABSTRACT FROM AUTHOR]

Published

2014

12. EST-SNP genotyping of citrus species using high-resolution melting curve analysis.

Author

Distefano, Gaetano, La Malfa, Stefano, Gentile, Alessandra, and Wu, Shu-Biao

Subjects

SINGLE nucleotide polymorphisms, PLANT species, MELTING points, CITRUS, HIGH resolution imaging, PLANT reproduction, BIOMARKERS

Abstract

Citrus taxonomy is very complex mainly due to specific aspects of its reproductive biology. A number of studies have been performed using various molecular markers in order to evaluate the level of genetic variability in Citrus. SNP markers have been used for genetic diversity assessment using a variety of different methods. Recently, the availability of EST database and whole genome sequences has made it possible to develop more markers such as SNPs. In the present study, the high-resolution melting curve analysis (HRM) was used to detect SNPs or INDELs in Citrus genus for the first time. We aimed to develop a panel of SNPs to differentiate Citrus genotypes which can also be applied to Citrus biodiversity studies. The results showed that 21 SNP containing markers produced distinct polymorphic melting curves among the Citrus spp. investigated through HRM analysis. It was proved that HRM is an efficient, cost-effective, and accurate method for discriminating citrus SNPs as well as a method to analyze more polymorphisms in a single PCR amplicon, representing a useful tool for genetic, biodiversity, and breeding studies. SNPs developed based on Citrus sinensis EST database showed a good transferability within the Citrus genus. Moreover, HRM analysis allowed the discrimination of citrus genotypes at specific level and the resulting genetic distance analysis clustered these genotypes into three main branches. The results suggested that the panel of SNP markers could be used in a variety of applications in citrus biodiversity assessment and breeding programs using HRM analysis. [ABSTRACT FROM AUTHOR]

Published

2013

13. Development of amplified consensus genetic markers in Taxodiaceae based on Cryptomeria japonica ESTs data.

Author

Lu, Yong-quan, Jia, Qing, and Tong, Zai-kang

Abstract

Amplified consensus genetic marker (ACGM) is a PCR-based marker technique that uses primers designed within conserved regions of coding sequences. After a comparison of Cryptomeria japonica and Arabidopsis ESTs to search for conserved sequences, 237 single e-PCR products were obtained. We randomly selected 110 candidate ACGM markers to test. Of the 110 candidate ACGM markers tested, 106 yielded stable and clear PCR products in C. japonica. We then tested the utility of these 106 primer pairs in 10 species, representing 7 genera of Taxodiaceae. The number of specific amplification primer pairs among those 10 species varied from 49 to 103 (or 46.2∼97.2%). The 106 primer pairs (ACGM loci) were high transferable to Cryptomeria fortunei Hooibrenk (97.2%) but were low in Metasequoia glyptostroboides (46.2%). The number of PCR bands per primer pair ranged from 1.06 to 1.15, which means that most of the ACGM primers can obtain a single band within these 10 Taxodiaceae species. In summary, our study shows that ACGM is a technique applicable for marker development even in species with limited sequence data. [ABSTRACT FROM AUTHOR]

Published

2013

14. Development and Validation of Single Nucleotide Polymorphisms (SNPs) Markers from Two Transcriptome 454-Runs of Turbot (Scophthalmus maximus) Using High-Throughput Genotyping.

Author

Vera, Manuel, Alvarez-Dios, Jose-Antonio, Fernandez, Carlos, Bouza, Carmen, Vilas, Roman, and Martinez, Paulino

Subjects

*SINGLE nucleotide polymorphisms, *PSETTA maxima, *IMMUNE response, *GONADS, *HARDY-Weinberg formula, *BONFERRONI correction

Abstract

The turbot (Scophthalmus maximus) is a commercially valuable flatfish and one of the most promising aquaculture species in Europe. Two transcriptome 454-pyrosequencing runs were used in order to detect Single Nucleotide Polymorphisms (SNPs) in genes related to immune response and gonad differentiation. A total of 866 true SNPs were detected in 140 different contigs representing 262,093 bp as a whole. Only one true SNP was analyzed in each contig. One hundred and thirteen SNPs out of the 140 analyzed were feasible (genotyped), while Ш were polymorphic in a wild population. Transition/transversion ratio (1.354) was similar to that observed in other fish studies. Unbiased gene diversity (He) estimates ranged from 0.060 to 0.510 (mean = 0.351), minimum allele frequency (MAF) from 0.030 to 0.500 (mean = 0.259) and all loci were in Hardy-Weinberg equilibrium after Bonferroni correction. A large number of SNPs (49) were located in the coding region, 33 representing synonymous and 16 non-synonymous changes. Most SNP-containing genes were related to immune response and gonad differentiation processes, and could be candidates for functional changes leading to phenotypic changes. These markers will be useful for population screening to look for adaptive variation in wild and domestic turbot. [ABSTRACT FROM AUTHOR]

Published

2013

15. Characterization and genomic annotation of polymorphic EST- SSR loci in L itopenaeus vannamei shrimp.

Author

Santos, Camilla A, Rossini, Bruno C, Marques, Carla G, Galetti, Pedro M, and Freitas, Patrícia D

Subjects

*WHITELEG shrimp, *GENOMICS, *BIOLOGY, *GENETIC polymorphisms, *MICROSATELLITE repeats

Abstract

In the present work, EST- SSR (expressed sequence tag-simple sequence repeat) loci were obtained by screening 45 000 ESTs from the Pacific white shrimp L itopenaeus vannamei, which was available in a database of the ShEST ( Shrimp EST Genome Project) consortium. Fifty-two of 600 EST- SSR loci were selected. From this total, 21 EST- SSRs were polymorphic among 40 individuals and had their gene products ascribed. Two to 20 alleles per locus were detected and the observed heterozygosity ranged from 0.15 to 0.86. Eight loci presented a significant heterozygote deficit after the Bonferroni correction, which was attributed to null alleles. Seven loci were able to have their protein products, molecular functions and biological processes determined. Our results are promising for future studies that relate the levels of these gene polymorphisms with different biological responses to stress in aquaculture. [ABSTRACT FROM AUTHOR]

Published

2012

16. Exploitation of a turbot ( Scophthalmus maximus L.) immune-related expressed sequence tag (EST) database for microsatellite screening and validation.

Author

NAVAJAS-PÉREZ, R., ROBLES, F., MOLINA-LUZÓN, M. J., De La HERRÁN, R., ÁLVAREZ-DIOS, J. A., PARDO, B. G., VERA, M., BOUZA, C., and MARTÍNEZ, P.

Subjects

*PSETTA maxima, *MICROSATELLITE repeats, *HETEROZYGOSITY, *FLATFISHES, *FISH germplasm, *GENE mapping, *ATLANTIC halibut, *FISHES

Abstract

In this study, we identified and characterized 160 microsatellite loci from an expressed sequence tag (EST) database generated from immune-related organs of turbot ( Scophthalmus maximus). A final set of 83 new polymorphic microsatellites were validated after the analysis of 40 individuals of Atlantic origin including both wild and farmed individuals. The allele number and the expected heterozygosity ranged from 2 to 18 and from 0.021 to 0.951, respectively. Evidences of null alleles at moderate-high frequencies were detected at six loci using population data. None of the analysed loci showed deviations from Mendelian segregation after the analysis of five full-sib families including approximately 92 individuals/family. The markers are used to consolidate the turbot genetic map, and because they are mostly EST-derived, they will be very useful for comparative genomic studies within flatfishes and with model fish species. Using an in silico approach, we detected significant homologies of microsatellite sequences with the EST databases of the flatfish species with highest genomic resources (Senegalese sole, Atlantic halibut, bastard halibut) in 31% of these turbot markers. The conservation of these microsatellites within Pleuronectiformes will pave the way for anchoring genetic maps of different species and identifying genomic regions related to productive traits. [ABSTRACT FROM AUTHOR]

Published

2012

17. Generation of a large-scale genomic resource for functional and comparative genomics in Liriodendron tulipifera L.

Author

Liang, Haiying, Ayyampalayam, Saravanaraj, Wickett, Norman, Barakat, Abdelali, Xu, Yi, Landherr, Lena, Ralph, Paula, Jiao, Yuannian, Xu, Tao, Schlarbaum, Scott, Ma, Hong, Leebens-Mack, James, and dePamphilis, Claude

Abstract

Liriodendron tulipifera L., a member of Magnoliaceae in the order Magnoliales, has been used extensively as a reference species in studies on plant evolution. However, genomic resources for this tree species are limited. We constructed cDNA libraries from ten different types of tissues: premeiotic flower buds, postmeiotic flower buds, open flowers, developing fruit, terminal buds, leaves, cambium, xylem, roots, and seedlings. EST sequences were generated either by 454 GS FLX or Sanger methods. Assembly of almost 2.4 million sequencing reads from all libraries resulted in 137,923 unigenes (132,905 contigs and 4,599 singletons). About 50% of the unigenes had significant matches to publically available plant protein sequences, representing a wide variety of putative functions. Approximately 30,000 simple sequence repeats were identified. More than 97% of the cell wall formation genes in the Cell Wall Navigator and the MAIZEWALL databases are represented. The cinnamyl alcohol dehydrogenase ( CAD) homologs identified in the L. tulipifera EST dataset showed different expression levels in the ten tissue types included in this study. In particular, the LtuCAD1 was found to partially recover the stiffness of the floral stems in the Arabidopsis thaliana CAD4 and CAD5 double mutant plants, of the LtuCAD1 in lignin biosynthesis. L. tulipifera genes have greater sequence similarity to homologs from other woody angiosperm species than to non-woody model plants. This large-scale genomic resour"HistryDatesce will be instrumental for gene discovery, cDNA microarray production, and marker-assisted breeding in L. tulipifera, and strengthen this species' role in comparative studies. [ABSTRACT FROM AUTHOR]

Published

2011

18. Identification of SSR loci in Betula luminifera using birch EST data.

Author

Lu, Yong-quan, Li, Hai-ying, Jia, Qing, Huang, Hua-hong, and Tong, Zai-kang

Abstract

Expressed sequence tags (ESTs) are generated from single-pass sequencing of randomly picked cDNA clones and can be used for development of simple sequence repeat (SSR) markers or microsatellites. However, EST databases have been developed for only a small number of species. This paper provides a case study of the utility of freely available birch EST resources for the development of markers necessary for the genetic analysis of Betula luminifera. Based on birch EST data, primers for 80 EST-SSR candidate loci were developed and tested in birch. Of these, 59 EST-SSR loci yielded single, stable and clear PCR products. We then tested the utility of those 59 markers in B. luminifera. The results showed 28 (47.6%) yielded stable and clear PCR products for at least one B. luminifera genotype. In addition, this study describes a rapid and inexpensive alternative for the development of SSRs in species with scarce available sequence data. [ABSTRACT FROM AUTHOR]

Published

2011

19. Validation of single nucleotide polymorphism (SNP) markers from an immune Expressed Sequence Tag (EST) turbot, Scophthalmus maximus, database

Author

Vera, Manuel, Álvarez-Dios, José Antonio, Millán, Adrián, Pardo, Belén G., Bouza, Carmen, Hermida, Miguel, Fernández, Carlos, de la Herrán, Roberto, Molina-Luzón, María Jesús, and Martínez, Paulino

Subjects

*GENETIC markers, *GENETIC polymorphisms, *NUCLEOTIDE sequence, *GENE expression, *PSETTA maxima, *FISH populations, *HARDY-Weinberg formula

Abstract

Abstract: An expressed sequence tag (EST) turbot database from immune tissues was tracked to identify and validate single nucleotide polymorphism (SNP) markers suitable for map construction and population analysis in turbot (Scophthalmus maximus). By means of a stringent bioinformatic tracking strategy, 341 contigs containing true SNPs were identified among the 1827 existing in the database. The number of true SNPs per contig ranged between one and 20 for most contigs analyzed. However, some contigs showed higher numbers (many of them presumed artifactual SNPs), as a result of the bioinformatics workflow used for database construction and SNP searching. Two hundred and four contigs containing between one and nine SNPs or representing genes of special relevance were included for validation. Seventy-seven out of 166 SNPs that were successfully amplified resulted polymorphic and were combined in multiplexes for high-throughput genotyping. A total of 47 transitions, 28 transversions and two indels were detected among polymorphic SNPs, C/T being the commonest (34) and G/T the least common (4) substitutions observed. This represented a transition/transversion ratio of 1.885, similar to that observed in other fish studies. Minimum Allele Frequencies of the 77 polymorphic SNPs ranged from 0.031 to 0.500 (mean: 0.228±0.015) and unbiased expected heterozygosity (He) from 0.063 to 0.529 (mean: 0.329±0.016). Only two SNP loci deviated from Hardy–Weinberg expectations and no pair of loci deviated from random genotypic associations after correction for multiple tests. Analysis of segregation in eight large turbot families showed that only four loci deviated from Mendelian segregation after Bonferroni correction. The same analysis detected the presence of null alleles at two SNPs in accordance with the high frequency of null alleles estimated at these loci from population data. Fifteen contigs containing polymorphic SNPs (19.5%) could not be annotated after screening public databases with AutoFACT. Among those annotated, 43 (55.8%) were located in the 3′ untranslated region and 19 (24.7%) in the coding region, nine representing synonymous and 10 non-synonymous substitutions. Most of these genes appeared related to immune response and constitute candidates for functional changes in the correspondent proteins leading to putative phenotypic changes. These SNPs are the first validated in Scophthalmus maximus, a species of high aquaculture relevance, and provide new genetic tools for genetic mapping and QTL identification, and for population structure and parentage analysis. [Copyright &y& Elsevier]

Published

2011

20. A pipeline for high throughput detection and mapping of SNPs from EST databases.

Author

Anithakumari, A. M., Tang, Jifeng, van Eck, Herman J., Visser, Richard G. F., Leunissen, Jack A. M., Vosman, Ben, and van der Linden, C. Gerard

Subjects

*GENETIC polymorphisms, *DATABASES, *GENE mapping, *PLANT genetics, *BIOINFORMATICS

Abstract

Single nucleotide polymorphisms (SNPs) represent the most abundant type of genetic variation that can be used as molecular markers. The SNPs that are hidden in sequence databases can be unlocked using bioinformatic tools. For efficient application of these SNPs, the sequence set should be error-free as much as possible, targeting single loci and suitable for the SNP scoring platform of choice. We have developed a pipeline to effectively mine SNPs from public EST databases with or without quality information using QualitySNP software, select reliable SNP and prepare the loci for analysis on the Illumina GoldenGate genotyping platform. The applicability of the pipeline was demonstrated using publicly available potato EST data, genotyping individuals from two diploid mapping populations and subsequently mapping the SNP markers (putative genes) in both populations. Over 7000 reliable SNPs were identified that met the criteria for genotyping on the GoldenGate platform. Of the 384 SNPs on the SNP array approximately 12% dropped out. For the two potato mapping populations 165 and 185 SNPs segregating SNP loci could be mapped on the respective genetic maps, illustrating the effectiveness of our pipeline for SNP selection and validation. [ABSTRACT FROM AUTHOR]

Published

2010

21. Rainbow Smelt ( Osmerus mordax) Genomic Library and EST Resources.

Author

Schalburg, K., Leong, J., Cooper, G., Robb, A., Beetz-Sargent, M., Lieph, R., Holt, R., Moore, R., Ewart, K., Driedzic, W., ten Hallers, B., Zhu, B., Jong, P., Davidson, W., and Koop, B.

Abstract

Genomic resources in rainbow smelt ( Osmerus mordax) enable us to examine the genome duplication process in salmonids and test hypotheses relating to the fate of duplicated genes. They further enable us to pursue physiological and ecological studies in smelt. A bacterial artificial chromosome library containing 52,410 clones with an average insert size of 146 kb was constructed. This library represents an 11-fold average coverage of the rainbow smelt ( O. mordax) genome. In addition, several complementary deoxyribonucleic acid libraries were constructed, and 36,758 sequences were obtained and combined into 12,159 transcripts. Over half of these transcripts have been identified, several of which have been associated with cold adaptation. These basic resources show high levels of similarity (86%) to salmonid genes and provide initial support for genome duplication in the salmonid ancestor. They also facilitate identification of genes important to fish and direct us toward new technologies for other studies in fish biology. [ABSTRACT FROM AUTHOR]

Published

2008

22. An EST database for Liriodendron tulipifera L. floral buds: the first EST resource for functional and comparative genomics in Liriodendron.

Author

Liang, Haiying, Carlson, John, Leebens-Mack, James, Wall, P., Mueller, Lukas, Buzgo, Matyas, Landherr, Lena, Hu, Yi, DiLoreto, D., Ilut, Daniel, Field, Dawn, Tanksley, Steven, Ma, Hong, and dePamphilis, Claude

Abstract

Liriodendron tulipifera L. was selected by the Floral Genome Project for identification of new genes related to floral diversity in basal angiosperms. A large, non-normalized cDNA library was constructed from premeiotic and meiotic floral buds and sequenced to generate a database of 9,531 high-quality expressed sequence tags. These sequences clustered into 6,520 unigenes, of which 5,251 were singletons, and 1,269 were in contigs. Homologs of genes regulating many aspects of flower development were identified, including those for organ identity and development, cell and tissue differentiation, and cell-cycle control. Almost 5% of the transcriptome consisted of homologs to known floral gene families. Homologs of most of the genes involved in cell-wall construction were also recovered. This provides a new opportunity for comparative studies in lignin biosynthesis, a trait of key importance in the evolution of land plants and in the utilization of fiber from economically important tree species, such as Liriodendron. Also of note is that 1,089 unigenes did not match any sequence in the public databases, including the complete genomes of Arabidopsis, rice, and Populus. Some of these novel genes might be unique in basal angiosperm species and, when better characterized, may be informative for understanding the origins of diverged gene families. Thus, the Liriodendron expressed sequence tag database and library will help bridge our understanding of the mechanisms of flower initiation and development that are shared among basal angiosperms, eudicots, and monocots, and provide new opportunities for comparative analysis of gene families across angiosperm species. [ABSTRACT FROM AUTHOR]

Published

2008

23. Molecular characterization and expression analysis of the Rab GTPase family in Vitis vinifera reveal the specific expression of a VvRabA protein.

Author

Abbal, Philippe, Pradal, Martine, Muniz, Lisa, Sauvage, Fran&çois-Xavier, Chatelet, Philippe, Ueda, Takashi, and Tesniere, Catherine

Subjects

*GUANOSINE triphosphatase, *GRAPES, *BERRIES, *GENOMES, *GENE mapping, *CHROMOSOMES

Abstract

As a first step to investigate whether Rab GTPases are involved in grape berry development, the Vitis vinifera EST and gene databases were searched for members of the VvRab family. The grapevine genome was found to contain 26 VvRabs that could be distributed into all of the eight groups described in the literature for model plants. Genetic mapping was successfully performed; VvRabs were mostly located on independent chromosomes, apart from eight that were located on the as yet unassigned portions of the genome clustered in the ChrUn_Random chromosome. Conserved and divergent regions between VvRab protein sequences were identified. Transcript expression of 11 VvRabs was analysed by real-time quantitative RT-PCR. Except for VvRabA5b, transcript expression was detected, in general, in all the organs investigated, but with different patterns. In grape berries, VvRab transcripts were expressed at all stages of fruit development, with different profiles, except in the case of members of the A family which displayed generally similar patterns. The response to growth regulators in cell cultures was generally specific to each VvRab, with a differential pattern of expression for ethylene, auxin, and abscisic acid according to the VvRab. Interestingly, and unexpectedly considering transcript expression, western blotting using a monoclonal antibody raised against AtRabA5c (ARA4) showed a specific expression in the exocarp of ripe grape berries, in all seven red and white berry varieties tested. By contrast, no expression was detected in any of the other organs or tissues investigated. This paper contains the first description of Rab GTPases in V. vinifera. The involvement of a specific VvRab in grape berry late development and the potential role of this Rab GTPase are discussed in relation to literature data. [ABSTRACT FROM PUBLISHER]

Published

2008

24. Generation and analysis of an Eucalyptus globulus cDNA library constructed from seedlings subjected to low temperature conditions.

Author

Rasmussen-Poblete, Susana, Valdés, Jorge, Gamboa, Maria Cecilia, Valenzuela, Pablo D. T., and Krauskopf, Erwin

Subjects

*CELLULOSE, *FORESTRY biotechnology, *LIGNINS, *TEMPERATURE, *EUCALYPTUS globulus, *SEEDLINGS, *BIOSYNTHESIS

Abstract

Eucalyptus globulus is the most important commercial temperate hardwood in the world because of its wood properties and due to its characteristics for biofuel production. However, only a very low number of expressed sequence tags (ESTs) are publicly available for this tree species. We constructed a cDNA from E. globulus seedlings subjected to low temperature and sequenced 9,913 randomly selected clones, generating 8,737 curated ESTs. The assembly produced 1,062 contigs and 3,879 singletons forming a Eucalyptus unigene set. Based on BLASTX analysis, 89.3% of the contigs and 88.5% of the singletons had significant similarity to known genes in the non-redundant database of GenBank. The Eucalyptus unigene set generated is a valuable public resource that provides an initial model for genes and regulatory pathways involved in cell wall biosynthesis at low temperature. [ABSTRACT FROM AUTHOR]

Published

2008

25. Molecular characterization and expression analysis of the Rop GTPase family in Vitis vinifera.

Author

Abbal, Philippe, Pradal, Martine, Sauvage, François-Xavier, Chatelet, Philippe, Paillard, Sophie, Canaguier, Aurélie, Adam-Blondon, Anne-Françoise, and Tesniere, Catherine

Subjects

*GUANOSINE triphosphatase, *GRAPES, *PROTEINS, *GENOMES, *PLANT physiology

Abstract

Rop/Rac GTPases are plant-specific signalling proteins with multiple roles, some of which have implications in plant development and in hormone signal transduction. Using expressed sequence tag (EST) and gene database analyses, members of the Rop family were characterized for the first time in a perennial species (Vitis vinifera). The grapevine genome was found to contain seven expressed VvRops. The phylogenetic analyses indicated that VvRops could be distributed into four groups, as described in the literature for model plants. Genetic mapping was successfully performed for five VvRops, which were localized on independent linkage groups. Conserved and divergent regions were identified on the protein sequences. The results of VvRop expression obtained by real-time quantitative reverse transcription-PCR analyses indicated that all the organs investigated displayed VvRop expression, however with different patterns. Whereas no total organ specificity for VvRop expression could be evidenced, VvRop9 displayed high expression in developing berries only. During berry development, the transcript profile was generally similar for all the VvRops, i.e. displaying a peak early in the herbaceous phase followed by a decline towards veraison and thereafter. Western blotting gave a similar expression profile for VvRop proteins. Response to growth regulators was generally specific to each VvRop. The potential involvement of specific VvRops in grapevine development is discussed. [ABSTRACT FROM PUBLISHER]

Published

2007

26. Functional study of hot pepper 26S proteasome subunit RPN7 induced by Tobacco mosaic virus from nuclear proteome analysis

Author

Lee, Boo-Ja, Kwon, Sun Jae, Kim, Sung-Kyu, Kim, Ki-Jeong, Park, Chang-Jin, Kim, Young-Jin, Park, Ohkmae K., and Paek, Kyung-Hee

Subjects

*CELL death, *GREEN fluorescent protein, *CELL nuclei, *ELECTROPHORESIS

Abstract

Abstract: Two-dimensional gel electrophoresis (2-DE) was applied for the screening of Tobacco mosaic virus (TMV)-induced hot pepper (Capsicum annuum cv. Bugang) nuclear proteins. From differentially expressed protein spots, we acquired the matched peptide mass fingerprint (PMF) data, analyzed by MALDI-TOF MS, from the non-redundant hot pepper EST protein FASTA database using the VEMS 2.0 software. Among six identified nuclear proteins, the hot pepper 26S proteasome subunit RPN7 (CaRPN7) was subjected to further study. The level of CaRPN7 mRNA was specifically increased during incompatible TMV–P0 interaction, but not during compatible TMV–P1.2 interaction. When CaRPN7::GFP fusion protein was targeted in onion cells, the nuclei had been broken into pieces. In the hot pepper leaves, cell death was exacerbated and genomic DNA laddering was induced by Agrobacterium-mediated transient overexpression of CaPRN7. Thus, this report presents that the TMV-induced CaRPN7 may be involved in programmed cell death (PCD) in the hot pepper plant. [Copyright &y& Elsevier]

Published

2006

27. Construction, database integration, and application of an Oenothera EST library

Author

Mráček, Jaroslav, Greiner, Stephan, Cho, Won Kyong, Rauwolf, Uwe, Braun, Martha, Umate, Pavan, Altstätter, Johannes, Stoppel, Rhea, Mlčochová, Lada, Silber, Martina V., Volz, Stefanie M., White, Sarah, Selmeier, Renate, Rudd, Stephen, Herrmann, Reinhold G., and Meurer, Jörg

Subjects

*OENOTHERA, *GENOMES, *GENETIC engineering, *LIBRARY automation

Abstract

Abstract: Coevolution of cellular genetic compartments is a fundamental aspect in eukaryotic genome evolution that becomes apparent in serious developmental disturbances after interspecific organelle exchanges. The genus Oenothera represents a unique, at present the only available, resource to study the role of the compartmentalized plant genome in diversification of populations and speciation processes. An integrated approach involving cDNA cloning, EST sequencing, and bioinformatic data mining was chosen using Oenothera elata with the genetic constitution nuclear genome AA with plastome type I. The Gene Ontology system grouped 1621 unique gene products into 17 different functional categories. Application of arrays generated from a selected fraction of ESTs revealed significantly differing expression profiles among closely related Oenothera species possessing the potential to generate fertile and incompatible plastid/nuclear hybrids (hybrid bleaching). Furthermore, the EST library provides a valuable source of PCR-based polymorphic molecular markers that are instrumental for genotyping and molecular mapping approaches. [Copyright &y& Elsevier]

Published

2006

28. ChickGCE: A novel germ cell EST database for studying the early developmental stage in chickens

Author

Kim, Heebal, Lim, Dajeong, Han, Beom Ku, Sung, Samsun, Jeon, Mina, Moon, Sunjin, Kang, Yeonkyung, Nam, Jungrye, and Han, Jae Yong

Subjects

*GERMPLASM, *HEREDITY, *GENITALIA, *SPERMATOGENESIS

Abstract

Abstract: We established a database to study germ cells during the early developmental stage in the chicken. The ChickGCE database provides integrated expressed sequence tag (EST) data from chicken testis, ovary, embryonic gonads, and primordial germ cells. We gathered data on 10,294 ESTs from approximately 1000 embryonic gonads, and we experimentally determined 10,851 ESTs from primordial germ cells purified from 7955 embryonic gonads by magnetically activated cell sorting. The EST testis and ovary datasets were retrieved from the public database of The Institute for Genomic Research (TIGR). The EST data were clustered and assembled into unique sequences, contigs, and singletons. The ChickGCE database provides functional annotation, identification, and putative embryonic germ-cell-specific novel transcripts based on the Gene Ontology database, as well as statistical analyses of expression patterns and pair-wise comparisons of two types of tissue- and germ-cell-specific alternative splicing events in the chicken. The new database is accessible online and queries can be answered using several search options, including tissue database searches, keywords, clone IDs, expected values, and BLAST search scores. [Copyright &y& Elsevier]

Published

2006

29. Reverse transcriptase template switching and false alternative transcripts

Author

Cocquet, Julie, Chong, Allen, Zhang, Guanglan, and Veitia, Reiner A.

Subjects

*REVERSE transcriptase, *HOMOLOGY (Biology), *DNA, *DNA polymerases

Abstract

Abstract: Reverse transcriptase (RT) can switch from one template to another in a homology-dependent manner. In the study of eukaryotic transcripts, this propensity of RT can produce an artificially deleted cDNA, which can be wrongly interpreted as an alternative transcript. Here, we have investigated the presence of such template-switching artifacts in cDNA databases, by scanning a collection of human splice sites (Information for the Coordinates of Exons, ICE database). We have confirmed several cases at the experimental level. Artifacts represent a significant portion of apparently spliced sequences using noncanonical splice signals but are rare in the context of the whole database. However, care should be taken in the annotation of alternative transcripts, especially when the RT used is poorly thermostable and when the putative intron is flanked by direct repeats, which are the substrate for template switching. [Copyright &y& Elsevier]

Published

2006

30. Identification of BCOX1, a novel gene overexpressed in breast cancer

Author

Song, Jin, Yang, Wanjun, Shih, Ie-Ming, Zhang, Zhen, and Bai, Jining

Subjects

*ANTIGENS, *EPITHELIAL cells, *MESSENGER RNA, *AMINO acids

Abstract

Abstract: The identification of tumor-associated antigens, which are specifically expressed in cancer tissues, is of utmost important for immunotherapy of breast cancer. We have combined in silico screening and experimental expression analysis to identify genes that are differentially expressed in breast carcinomas compared with their corresponding normal tissues. Using these approaches, we identified a novel gene, BCOX1, with overexpression in breast carcinoma. BCOX1 was highly homologous to KIAA0100, a hypothetical gene located on chromosome 17q11.2. RNA in situ hybridization shows that BCOX1 mRNA signal is mainly located in the cytoplasm of breast carcinoma epithelial cells, but not in those of normal epithelial cells, stroma cells and lymphocytes. Furthermore, mRNA expression of BCOX1 was moderately elevated in ductal in situ carcinoma (DCIS), peaked in invasive breast carcinoma (IBC) and metastatic breast carcinoma cells (MET) whereas absent in benign ductal epithelial cells. The predicted BCOX1 open reading frame of 666 bp encodes a putative protein of 222 amino acid residues with a calculated molecular weight of 24920 Da and a PI of 5.86. Computational analyses predict that the putative BCOX1 protein is a cytoplasmic protein. The functional relevance of this novel gene is yet to be determined. This study warrants further investigations to explore the molecular functions of BCOX1, and to determine its potential diagnostic and therapeutic applications for breast cancer. [Copyright &y& Elsevier]

Published

2006

31. Cloning and Alternative Splicing Analysis of Bombyx mori Transformer-2 Gene using Silkworm EST Database.

Author

Bao-Long Niu, Zhi-Qi Meng, Yue-Zhi Tao, Shun-Lin Lu, Hong-Biao Weng, Li-Hua He, and Wei-Feng Shen

Subjects

SILKWORMS, DNA, NUCLEOTIDE sequence, EXONS (Genetics), INTRONS, POLYMERASE chain reaction

Abstract

We have identified Bombyx mori transformer-2 gene ( Bmtra-2) cDNA by blasting the EST database of B. mori. It was expressed in the whole life of the male and female silkworm and was observed as a band of 1.3 kb by Northern blot analysis. By comparing corresponding ESTs to the Bmtra-2 DNA sequence, it was revealed that there were eight exons and seven introns, and all splice sites of exons/introns conformed to the GT/AG rule. Bmtra-2 pre-mRNA can produce multiple mRNAs encoding six distinct isoforms of BmTRA-2 protein using an alternative splicing pathway during processing. Six types of Bmtra-2 cDNA clones were identified by reverse transcription-polymerase chain reaction. All isoforms of BmTRA-2 protein contain two arginine/serine-rich domains and one RNA recognition motif, showing striking organizational similarity to Drosophila TRA-2 proteins. Edited by Zu-Xum GONG [ABSTRACT FROM AUTHOR]

Published

2005

32. Moss (Physcomitrella patens) functional genomics -- Gene discovery and tool development, with implications for crop plants and human health.

Author

Reski, Ralf and Frank, Wolfgang

Subjects

*MOSSES, *GENOMICS, *CROPS, *PHANEROGAMS, *GENES

Abstract

Recently, the moss Physcomitrella patens was established as a versatile tool in plant functional genomics. Mosses represent the oldest living clade of land plants, separated by approximately 450 million years of evolution from crop plants. Consequently, mosses contain metabolites and genes not known from these seed plants. In Physcomitrella, nuclear genes can be targeted by homologous recombination as efficiently as in yeast, allowing reverse genetics approaches in plants at high-throughput levels for the first time. Comprehensive expressed sequence tag databases gave new insights into the levels of diversity in land plants which are now ready to be exploited in plant biotechnology. In forward genetics screens, saturated tagged mutant collections help to unravel novel gene -- function relationships. Additionally, proteomics tools are at hand to analyse subcellular proteomes, as well as the phosphoproteome, as the core of eukaryotic signal transduction. Moreover, specifically designed Physcomitrella strains can produce human therapeutic proteins safely and cost-effectively in bioreactors. [ABSTRACT FROM AUTHOR]

Published

2005

33. THE GENETICS AND GENOMICS OF THE SILKWORM, BOMBYX MORI.

Author

Goldsmith, Marian R., Shimada, Toru, and Abe, Hiroaki

Subjects

*SILKWORMS, *CATERPILLARS, *LEPIDOPTERA, *INSECTS, *RNA, *GENETICS, *LINKAGE (Genetics)

Abstract

We review progress in applying molecular genetic and genomic technologies to studies in the domesticated silkworm, Bombyx mori, highlighting its use as a model for Lepidoptera, and in sericulture and biotechnology. Dense molecular linkage maps are being integrated with classical linkage maps for positional cloning and marker-assisted selection. Classical mutations have been identified by a candidate gene approach. Cytogenetic and sequence analyses show that the W chromosome is composed largely of nested full-length long terminal repeat retrotransposons. Z-chromosome-linked sequences show a lack of dosage compensation. The downstream sex differentiation mechanism has been studied via the silkworm homolog of doublesex. Expressed sequence tagged databases have been used to discover Lepidoptera-specific genes, provide evidence for horizontal gene transfer, and construct microarrays. Physical maps using large-fragment bacterial artificial chromosome libraries have been constructed, and whole-genome shotgun sequencing is underway. Germline transformation and transient expression systems are well established and available for functional studies, high-level protein expression, and gene silencing via RNA interference. [ABSTRACT FROM AUTHOR]

Published

2005

34. Microarray analysis of gene expression profiles in wing discs of Bombyx mori during pupal ecdysis

Author

Ote, Manabu, Mita, Kazuei, Kawasaki, Hideki, Seki, Motoaki, Nohata, Junko, Kobayashi, Masahiko, and Shimada, Toru

Subjects

*GENE expression, *SILKWORMS, *ECDYSTEROIDS, *ECDYSIS

Abstract

Wing discs of holometabolous insects undergo dramatic morphological changes during metamorphosis, a process that is controlled by the actions of hundreds of gene products. Using cDNA microarrays constructed from 5086 ESTs, we monitored the gene expression profiles in wing discs of Bombyx mori at 13 time points during pupal ecdysis (day-4 fifth instar larvae to day-0 pupae). Of the 5086 ESTs on the microarrays, 2998 ESTs had significant signals in more than half of the experiments. Of the 2998 ESTs, genes represented by 683 ESTs showed significant perturbations during pupal ecdysis. Genes previously known to be induced during metamorphosis were identified, including E75, Urbain, Chitinases, and cuticle proteins. The expressions of genes represented by 59 ESTs induced at the beginning of wandering contained genes predicted to be involved in protein degradation, amino acid metabolism, and amino acid transport. The expressions of genes represented by 147 ESTs induced after the ecdysteroid peak had a role in cuticle synthesis, pigmentation, ion transport, protein transport, and transcription regulation. The expressions of genes represented by 85 ESTs repressed after the ecdysteroid peak were predicted to be involved in nucleotide and nucleic acid metabolism and cell cycle. This indicates the involvement of several biological processes in wing disc development during metamorphosis. [Copyright &y& Elsevier]

Published

2004

35. TEPP, a new gene specifically expressed in testis, prostate, and placenta and well conserved in chordates

Author

Bera, Tapan Kumar, Hahn, Yoonsoo, Lee, Byungkook, and Pastan, Ira H.

Subjects

*GENE expression, *TESTIS, *PROSTATE cancer, *TISSUES

Abstract

We have combined computer-based screening and experimental expression analysis to identify genes that are expressed in normal prostate and/or prostate cancer but not in essential human tissues. Using this approach we identified a new gene that is specifically expressed in testis, prostate, and placenta. The gene has one major transcript of 1.0 kb in size and encodes for a protein of 30.7 kDa molecular weight. We named this gene TEPP (expressed in testis, prostate, and placenta). The amino acid sequence analysis of TEPP using SignalP program shows that it has a signal peptide with a predicted cleavage site between amino acids 19 and 20, indicating that it might be a secreted protein. Analysis of the predicted TEPP orthologs from different species shows that these proteins are highly conserved in chordates. In addition we have identified a splice variant of TEPP, which encodes a 37 kDa protein. In conclusion, a combination of bioinformatic and molecular approaches is useful in the identification of genes expressed in specific tissues. Selective expression of TEPP in testis, prostate, and in placenta and its high conservation among different species indicate that TEPP might have a role in reproductive biology. [Copyright &y& Elsevier]

Published

2003

36. Expanding our understanding of immunoglobulin, T-cell antigen receptor, and novel immune-type receptor genes: a subset of the immunoglobulin gene superfamily.

Author

Hawke, N. A., Yoder, J. A., and Litman, G. W.

Abstract

The immunoglobulin superfamily (IgSF) is an extensively diversified multigene family whose members share a common structural feature, the Ig fold. Members of the Ig/T-cell antigen receptor (TCR) subset of the IgSF mediate antigen-specific recognition in adaptive immune responses. Antigen-binding receptors belonging to this subset are present in all species of jawed vertebrates. To explore whether there are additional structurally related but otherwise distinct members of this subset, we have developed a technique termed the short-primer polymerase chain reaction (PCR) that targets structurally conserved short motifs in the Ig fold. Large-scale sequencing efforts and recent advances in information biotechnology, including "electronic PCR," provide additional computational means to implement similarly directed searches within databases. The use of these approaches has led to the discoveries of Ig/TCR homologues in a variety of phylogenetically diverse organisms, a diversified family of novel immune-type receptor genes, as well as a novel human IgSF member. The potential of random sequencing efforts and virtual screening of databases is described in the context of two novel genes in bony fish. The various methodologies that are discussed and the examples shown provide means for further investigating, and/or elucidating novel, IgSF receptors as well as components of pathways that are involved in immune responses in both traditional and nontraditional model systems. [ABSTRACT FROM AUTHOR]

Published

1999

37. Digital Cloning: Identification of Human cDNAs Homologous to Novel Kinases through Expressed Sequence Tag Database Searching.

Author

Chen, Hua-Chien, Kung, Hsing-Jien, and Robinson, Dan

Subjects

*HUMAN cloning, *GENETIC engineering, *ASEXUAL reproduction, *ANTISENSE DNA, *GENE expression, *NUCLEOTIDE sequence, *DATABASE searching

Abstract

Identification of novel kinases based on their sequence conservation within kinase catalytic domain has relied so far on two major approaches, low-stringency hybridization of cDNA libraries, and PCR method using degenerate primers. Both of these approaches at times are technically difficult and time-consuming. We have developed a procedure that can significantly reduce the time and effort involved in searching for novel kinases and increase the sensitivity of the analysis. This procedure exploits the computer analysis of a vast resource of human cDNA sequences represented in the expressed sequence tag (EST) database. Seventeen novel human cDNA clones showing significant homology to serine/threonine kinases, including STE-20, CDK- and YAK-related family kinases, were identified by searching EST database. Further sequence analysis of these novel kinases obtained either directly from EST clones or from PCR-RACE products confirmed their identity as protein kinases. Given the rapid accumulation of the EST database and the advent of powerful computer analysis software, this approach provides a fast, sensitive, and economical way to identify novel kinases as well as other genes from EST database. [ABSTRACT FROM AUTHOR]

Published

1998

38. Development of a panel of unigene-derived polymorphic EST–SSR markers in lentil using public database information

Author

Shiv Kumar, Debjyoti Sen Gupta, Clarice J. Coyne, Michael Baum, Pushparajah Thavarajah, Dil Thavarajah, Gaurav Sablok, Rebecca J. McGee, and Peng Cheng

Subjects

0106 biological sciences, 0301 basic medicine, Lens culinaris, UniGene, Settore BIO/03 - BOTANICA AMBIENTALE E APPLICATA, Plant Science, Biology, computer.software_genre, 01 natural sciences, lcsh:Agriculture, 03 medical and health sciences, Annotation, EST database, lcsh:Agriculture (General), Genome size, Genetic resources, Comparative genomics, Genetics, Expressed sequence tag, Database, Unigene sequences, lcsh:S, food and beverages, Functional annotation, lcsh:S1-972, 030104 developmental biology, Genetic marker, EST–SSRs, Microsatellite, UniProt, Agronomy and Crop Science, computer, 010606 plant biology & botany

Abstract

Lentil ( Lens culinaris Medik.), a diploid (2 n = 14) with a genome size greater than 4000 Mbp, is an important cool season food legume grown worldwide. The availability of genomic resources is limited in this crop species. The objective of this study was to develop polymorphic markers in lentil using publicly available curated expressed sequence tag information (ESTs). In this study, 9513 ESTs were downloaded from the National Center for Biotechnology Information (NCBI) database to develop unigene-based simple sequence repeat (SSR) markers. The ESTs were assembled into 4053 unigenes and then analyzed to identify 374 SSRs using the MISA microsatellite identification tool. Among the 374 SSRs, 26 compound SSRs were observed. Primer pairs for these SSRs were designed using Primer3 version 1.14. To classify the functional annotation of ESTs and EST–SSRs, BLASTx searches (using E-value 1 × 10 − 5 ) against the public UniProt ( http://www.uniprot.org /) and NCBI ( http://www.ncbi.nlh.nih.gov /) databases were performed. Further functional annotation was performed using PLAZA (version 3.0) comparative genomics and GO annotation was summarized using the Plant GO slim category. Among the synthesized 312 primers, 219 successfully amplified Lens DNA. A diverse panel of 24 Lens genotypes was used to identify polymorphic markers. A polymorphic set of 57 markers successfully discriminated the test genotypes. This set of polymorphic markers with functional annotation data could be used as molecular tools in lentil breeding.

Published

2016

39. A pipeline for high throughput detection and mapping of SNPs from EST databases

Author

C. Gerard van der Linden, Jifeng Tang, Ben Vosman, Herman J. van Eck, Jack A. M. Leunissen, Richard G. F. Visser, and A. M. Anithakumari

Subjects

construction, haplotype, Bioinformatics, markers, Single-nucleotide polymorphism, Plant Science, Biology, computer.software_genre, Molecular Inversion Probe, Article, Illumina GoldenGate assay, Laboratorium voor Plantenveredeling, Gene mapping, EST database, PRI Biodiversiteit en Veredeling, single-nucleotide polymorphisms, Bioinformatica, Genetics, SNP, genome, Molecular Biology, Genotyping, Database, EPS-3, QualitySNP, linkage maps, map-based cloning, food and beverages, Tag SNP, SNP genotyping, PRI Biodiversity and Breeding, Plant Breeding, varieties, potato, Agronomy and Crop Science, computer, discovery, Biotechnology, SNP array

Abstract

Single nucleotide polymorphisms (SNPs) represent the most abundant type of genetic variation that can be used as molecular markers. The SNPs that are hidden in sequence databases can be unlocked using bioinformatic tools. For efficient application of these SNPs, the sequence set should be error-free as much as possible, targeting single loci and suitable for the SNP scoring platform of choice. We have developed a pipeline to effectively mine SNPs from public EST databases with or without quality information using QualitySNP software, select reliable SNP and prepare the loci for analysis on the Illumina GoldenGate genotyping platform. The applicability of the pipeline was demonstrated using publicly available potato EST data, genotyping individuals from two diploid mapping populations and subsequently mapping the SNP markers (putative genes) in both populations. Over 7000 reliable SNPs were identified that met the criteria for genotyping on the GoldenGate platform. Of the 384 SNPs on the SNP array approximately 12% dropped out. For the two potato mapping populations 165 and 185 SNPs segregating SNP loci could be mapped on the respective genetic maps, illustrating the effectiveness of our pipeline for SNP selection and validation. ELECTRONIC SUPPLEMENTARY MATERIAL: The online version of this article (doi:10.1007/s11032-009-9377-5) contains supplementary material, which is available to authorized users.

Published

2010

40. Molecular characterization and expression analysis of the Rab GTPase family in Vitis vinifera reveal the specific expression of a VvRabA protein

Author

Catherine Tesniere, Takashi Ueda, Martine Pradal, Philippe Abbal, Philippe Chatelet, François-Xavier Sauvage, Lisa Muniz, Sciences Pour l'Oenologie (SPO), Institut national d’études supérieures agronomiques de Montpellier (Montpellier SupAgro), Institut national d'enseignement supérieur pour l'agriculture, l'alimentation et l'environnement (Institut Agro)-Institut national d'enseignement supérieur pour l'agriculture, l'alimentation et l'environnement (Institut Agro)-Université Montpellier 1 (UM1)-Université de Montpellier (UM)-Institut National de la Recherche Agronomique (INRA), Développement et amélioration des plantes (UMR DAP), Centre de Coopération Internationale en Recherche Agronomique pour le Développement (Cirad)-Institut National de la Recherche Agronomique (INRA)-Université Montpellier 2 - Sciences et Techniques (UM2)-Centre National de la Recherche Scientifique (CNRS), and The University of Tokyo (UTokyo)

Subjects

0106 biological sciences, Physiology, Arabidopsis, Gene Expression, Plant Science, GTPase, TRANSCRIPT LEVEL, UNIGENE CLUSTERING, 01 natural sciences, Genome, Gene Expression Regulation, Plant, Vitis, Cells, Cultured, Conserved Sequence, Phylogeny, Plant Proteins, Genetics, chemistry.chemical_classification, 0303 health sciences, RAB GTPASE, Chromosome Mapping, Gene Expression Regulation, Developmental, food and beverages, [SDV.BV.BOT]Life Sciences [q-bio]/Vegetal Biology/Botanics, EST DATABASE, White (mutation), Multigene Family, Genome, Plant, DNA, Complementary, QUANTITATIVE RT-PCR, Molecular Sequence Data, Biology, FRUIT RIPENING, 03 medical and health sciences, Gene mapping, Auxin, BIOLOGIE DU DEVELOPPEMENT, Amino Acid Sequence, Gene, 030304 developmental biology, fungi, Chromosome, Molecular biology, GENOME MAPPING, chemistry, rab GTP-Binding Proteins, Rab, Plant Structures, Sequence Alignment, 010606 plant biology & botany

Abstract

International audience; As a first step to investigate whether Rab GTPases are involved in grape berry development, the Vitis vinifera EST and gene databases were searched for members of the VvRab family. The grapevine genome was found to contain 26 VvRabs that could be distributed into all of the eight groups described in the literature for model plants. Genetic mapping was successfully performed; VvRabs were mostly located on independent chromosomes, apart from eight that were located on the as yet unassigned portions of the genome clustered in the ChrUn_Random chromosome. Conserved and divergent regions between VvRab protein sequences were identified. Transcript expression of 11 VvRabs was analysed by real-time quantitative RT-PCR. Except for VvRabA5b, transcript expression was detected, in general, in all the organs investigated, but with different patterns. In grape berries, VvRab transcripts were expressed at all stages of fruit development, with different profiles, except in the case of members of the A family which displayed generally similar patterns. The response to growth regulators in cell cultures was generally specific to each VvRab, with a differential pattern of expression for ethylene, auxin, and abscisic acid according to the VvRab. Interestingly, and unexpectedly considering transcript expression, western blotting using a monoclonal antibody raised against AtRabA5c (ARA4) showed a specific expression in the exocarp of ripe grape berries, in all seven red and white berry varieties tested. By contrast, no expression was detected in any of the other organs or tissues investigated. This paper contains the first description of Rab GTPases in V. vinifera. The involvement of a specific VvRab in grape berry late development and the potential role of this Rab GTPase are discussed in relation to literature data

Published

2008

41. Genotyping and Mutation Scanning by High Resolution Melting (HRM) Analysis of Citrus EST-SNPs and SSRs

Author

Distefano, Gaetano, LO PIERO, Angela Roberta, LA MALFA, Stefano Giovanni, Caruso, M., Nicolosi, Elisabetta, Wu, S., and Gentile, Alessandra

Subjects

Citrus, EST database, high resolution melting curve

Published

2015

42. Construction, database integration, and application of an Oenothera EST library

Author

Martha Braun, Stefanie M. Volz, Stephen Rudd, Stephan Greiner, Lada Mlcòchová, Reinhold G. Herrmann, Jörg Meurer, Pavan Umate, Jaroslav Mráček, Sarah White, Johannes Altstätter, Rhea Stoppel, Renate Selmeier, Uwe Rauwolf, Won Kyong Cho, and Martina V. Silber

Subjects

Genetic Markers, Plant Infertility, Nuclear gene, food.ingredient, Oenothera, Genomics, Computational biology, Biology, Oenothera elata, Genome, chemistry.chemical_compound, food, Eukaryotic genome evolution, EST database, Molecular evolution, Molecular marker, Genetics, Plastids, Expression profiling, Codominant molecular marker, Gene Library, Cell Nucleus, Expressed Sequence Tags, Interspecific genome/plastome hybrids and cybrids, Chromosome Mapping, biology.organism_classification, Gene expression profiling, chemistry, Genome/plastome incompatibility

Abstract

Coevolution of cellular genetic compartments is a fundamental aspect in eukaryotic genome evolution that becomes apparent in serious developmental disturbances after interspecific organelle exchanges. The genus Oenothera represents a unique, at present the only available, resource to study the role of the compartmentalized plant genome in diversification of populations and speciation processes. An integrated approach involving cDNA cloning, EST sequencing, and bioinformatic data mining was chosen using Oenothera elata with the genetic constitution nuclear genome AA with plastome type I. The Gene Ontology system grouped 1621 unique gene products into 17 different functional categories. Application of arrays generated from a selected fraction of ESTs revealed significantly differing expression profiles among closely related Oenothera species possessing the potential to generate fertile and incompatible plastid/nuclear hybrids (hybrid bleaching). Furthermore, the EST library provides a valuable source of PCR-based polymorphic molecular markers that are instrumental for genotyping and molecular mapping approaches.

Published

2006

43. terMITEs: miniature inverted-repeat transposable elements (MITEs) in the termite genome (Blattodea: Termitoidae)

Author

Andrea Luchetti and Luchetti, A.

Subjects

Transposable element, Inverted repeat, Random genomic library, Genome, Insect, Molecular Sequence Data, Isoptera, Biology, Genome, DNA sequencing, Tandem repeat, Phylogenetics, EST database, Termite, Genetics, Animals, Copy-number variation, Molecular Biology, Phylogeny, Base Sequence, Inverted Repeat Sequences, Genetic Variation, General Medicine, Miniature inverted-repeat transposable element (MITE), Mutagenesis, Insertional, DNA Transposable Elements, Insect Proteins, Tandem exon duplication

Abstract

Transposable elements (TEs) are discrete DNA sequences which are able to replicate and jump into different genomic locations. Miniature inverted-repeats TEs (MITEs) are non-autonomous DNA elements whose origin is still poorly understood. Recently, some MITEs were found to contain core repeats that can be arranged in tandem arrays; in some instances, these arrays have even given rise to satellite DNAs in the (peri)centromeric region of the host chromosomes. I report the discovery and analysis of three new MITEs found in the genome of several termite species (hence the name terMITEs) in two different families. For two of the MITEs (terMITE1-Tc1/mariner superfamily; terMITE2-piggyBac superfamily), evidence of past mobility was retrieved. Moreover, these two MITEs contained core repeats, 16 bp and 114 bp long respectively, exhibiting copy number variation. In terMITE2, the tandem duplication appeared associated with element degeneration, in line with a recently proposed evolutionary model on MITEs and the origin of tandem arrays. Concerning their genomic distribution, terMITE1 and terMITE3 appeared more frequently inserted close to coding regions while terMITE2 was mostly associated with TEs. Although MITEs are commonly distributed in coding regions, terMITE2 distribution is in line with that of other insects' piggyBac-related elements and of other small TEs found in termite genomes. This has been explained through insertional preference rather than through selective processes. Data presented here add to the knowledge on the poorly exploited polyneopteran genomes and will provide an interesting framework in which to study TEs' evolution and host's life history traits.

Published

2014

44. A legume genomics resource: The Chickpea Root Expressed Sequence Tag Database

Author

Jonathan H. Crouch, Sanjeev Shinde, Hutokshi K. Buhariwalla, and B. Jayashree

Subjects

Expressed sequence tag, Resource (biology), drought avoidance, Database, biology, fungi, Drought tolerance, cloning, drought tolerance, food and beverages, Genomics, data mining, computer.software_genre, biology.organism_classification, Applied Microbiology and Biotechnology, Genome, Medicago truncatula, Crop, stress, root traits, Agronomy, EST database, computer, Legume, Biotechnology

Abstract

Chickpea, a lesser-studied grain legume, is being investigated due to its taxonomic proximity with the model legume genome Medicago truncatula and its ability to endure and grow in relatively low soil water contents making it a model legume crop for the study of agronomic response to drought stress. Public databases currently contain very few sequences from chickpea associated with expression in root tissues. However, root traits are likely to be one of the most important components of drought tolerance in chickpea. Thus, we have generated a set of over 2800 chickpea expressed sequence tags (ESTs) from a library constructed after subtractive suppressive hybridization (SSH) of root tissue from two closely related chickpea genotypes possessing different sources of drought avoidance and tolerance (ICC4958 and Annigeri respectively). This database provides researchers in legume genomics with a major new resource for data mining associated with root traits and drought tolerance. This report describes the development and utilization of the database and provides the tools we have developed to facilitate the bioinformatics pipeline used for analysis of the ESTs in this database. We also discuss applications that have already been achieved using this resource.

Published

2005

45. EST database for early flower development in California poppy (Eschscholzia californica Cham., Papaveraceae) tags over 6000 genes from a basal eudicot

Author

Carlson, John E., Leebens-Mack, James H., Wall, P. Kerr, Zahn, Laura M., Mueller, Lukas A., Landherr, Lena L., Hu, Yi, Ilut, Daniel C., Arrington, Jennifer M., Choirean, Stephanie, Becker, Annette, Field, Dawn, Tanksley, Steven D., Ma, Hong, and dePamphilis, Claude W.

Published

2006

46. Physiological and proteomic analyses of salt stress response in the halophyte Halogeton glomeratus

Author

Meng Yaxiong, Wang Huajun, Yang Ke, Xu Xianliang, Wang Juncheng, Ma Xiaole, Xunwu Shang, Si Erjing, Yong Lai, Di Wang, and Li Baochun

Subjects

Proteomics, Proteome, medicine.medical_treatment, Sodium, chemistry.chemical_element, Plant Science, Chenopodiaceae, Sodium Chloride, Photosynthesis, Plant Roots, salinity, Stress, Physiological, Tandem Mass Spectrometry, EST database, Halophyte, Botany, medicine, Cluster Analysis, Saline, proteomic, Plant Proteins, tolerance, biology, Plant Stems, Salt-Tolerant Plants, Salt Tolerance, Original Articles, Halogeton glomeratus, biology.organism_classification, Salinity, Plant Leaves, chemistry, Seedling, Seedlings, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Plant Stomata, physiology

Abstract

Very little is known about the adaptation mechanism of Chenopodiaceae Halogeton glomeratus, a succulent annual halophyte, under saline conditions. In this study, we investigated the morphological and physiological adaptation mechanisms of seedlings exposed to different concentrations of NaCl treatment for 21 d. Our results revealed that H. glomeratus has a robust ability to tolerate salt; its optimal growth occurs under approximately 100 mm NaCl conditions. Salt crystals were deposited in water-storage tissue under saline conditions. We speculate that osmotic adjustment may be the primary mechanism of salt tolerance in H. glomeratus, which transports toxic ions such as sodium into specific salt-storage cells and compartmentalizes them in large vacuoles to maintain the water content of tissues and the succulence of the leaves. To investigate the molecular response mechanisms to salt stress in H. glomeratus, we conducted a comparative proteomic analysis of seedling leaves that had been exposed to 200 mm NaCl for 24 h, 72 h and 7 d. Forty-nine protein spots, exhibiting significant changes in abundance after stress, were identified using matrix-assisted laser desorption ionization tandem time-of-flight mass spectrometry (MALDI-TOF/TOF MS/MS) and similarity searches across EST database of H. glomeratus. These stress-responsive proteins were categorized into nine functional groups, such as photosynthesis, carbohydrate and energy metabolism, and stress and defence response.

Published

2014

47. Trichoplaxin - A new membrane-active antimicrobial peptide from placozoan cDNA

Author

Monica Benincasa, Juraj Simunić, Dražen Petrov, Nédia Kamech, Tahar Bouceba, Davor Juretić, Ingénierie des protéines, PCR, Interaction Moléculaires [IBPS] (IBPS-IPIM), Institut de Biologie Paris Seine (IBPS), Université Pierre et Marie Curie - Paris 6 (UPMC)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Centre National de la Recherche Scientifique (CNRS)-Université Pierre et Marie Curie - Paris 6 (UPMC)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Centre National de la Recherche Scientifique (CNRS), Croatian Ministry of Science, Education and Sports [177-1770495-0476], French government, Institut National de la Santé et de la Recherche Médicale (INSERM)-Université Pierre et Marie Curie - Paris 6 (UPMC)-Centre National de la Recherche Scientifique (CNRS)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Université Pierre et Marie Curie - Paris 6 (UPMC)-Centre National de la Recherche Scientifique (CNRS), Simunić, Juraj, Petrov, Dražen, Bouceba, Tahar, Kamech, Nédia, Benincasa, Monica, and Juretić, Davor

Subjects

Anti-Infective Agent, Secondary, [SDV]Life Sciences [q-bio], Peptide, Biochemistry, Protein Structure, Secondary, chemistry.chemical_compound, Anti-Infective Agents, EST database, Models, Complementary, Candida, chemistry.chemical_classification, Expressed sequence tag, Antimicrobial Cationic Peptide, Tumor, Membrane, Bacterial, U937 Cells, Antimicrobial, Peptide–membrane interaction, U937 Cell, Antimicrobial peptide, Lead compound, Peptide-membrane interaction, Trichoplax adhaeren, Human, Signal peptide, DNA, Bacterial, Protein Structure, DNA, Complementary, Molecular Sequence Data, Biophysics, Biology, Gram-Positive Bacteria, Models, Biological, Cell Line, Complementary DNA, Cell Line, Tumor, Surface plasmon resonance, Gram-Negative Bacteria, Animals, Humans, Placozoa, Propidium iodide, Amino Acid Sequence, antimicrobial peptide, Trichoplax adhaerens, selectivity index, surface plasmon resonance, peptide-membrane interaction, Kinetic, Membranes, Animal, DNA, Cell Biology, Selectivity index, Biological, Molecular biology, Antimicrobial Cationic Peptides, Kinetics, Rats, Sequence Alignment, Surface Plasmon Resonance, chemistry, Rat

Abstract

International audience; A method based on the use of signal peptide sequences from antimicrobial peptide (AMP) precursors was used to mine a placozoa expressed sequence tag database and identified a potential antimicrobial peptide from Trichoplax adhaerens. This peptide, with predicted sequence FFGRLKSVWSAVKHGWKAAKSR is the first AMP from a placozoan species, and was named trichoplaxin. It was chemically synthesized and its structural properties, biological activities and membrane selectivity were investigated. It adopts an a-helical structure in contact with membrane-like environments and is active against both Gram-negative and Gram-positive bacterial species (including MRSA), as well as yeasts from the Candida genus. The cytotoxic activity, as assessed by the haemolytic activity against rat erythrocytes, U937 cell permeabilization to propidium iodide and MCF7 cell mitochondrial activity, is significantly lower than the antimicrobial activity. In tests with membrane models, trichoplaxin shows high affinity for anionic prokaryote-like membranes with good fit in kinetic studies. Conversely, there is a low affinity for neutral eukaryote-like membranes and absence of a dose dependent response. With high selectivity for bacterial cells and no homologous sequence in the UniProt, trichoplaxin is a new potential lead compound for development of broad-spectrum antibacterial drugs.

Published

2014

48. Tobacco by-2 cells: The present and beyond

Author

Nagata, Toshiyuki, Sakamoto, Kenichi, and Shimizu, Takashi

Published

2004

49. Identification, conservation, and relative expression of V-ATPase cDNAs in tomato plants

Author

Coker, Jeffrey S., Jones, Derek, and Davies, Eric

Published

2003

50. cDNA Cloning of the Putative Human β-1,4 Mannosyltransferase Gene which is Involved in Lipid-linked Oligosaccharide Synthesis

Subjects

Glycosylation, EST database, Lipid-linked oligosaccharide, cDNA cloning, Mannosyltransferase

Published

1998