Isolation of the transposable element hupfer from the entomopathogenic fungus Beauveria bassiana by insertion mutagenesis of the nitrate reductase structural gene

A transposable element has been isolated from the entomopathogenic fungus Beauveria bassiana by trapping it in the nitrate reductase structural gene, which has been cloned from this species. The element had inserted in the first exon of the nia gene and appeared to have duplicated the sequence TA at the site of insertion. It was 3336?bp long with 30-bp imperfect, inverted, terminal repeats. The element, called hupfer, contained an open reading frame encoding a 321-amino acid protein similar to the IS630- or mariner-Tc1-like transposases, and a residual sequence of about 2?kb which was not significantly similar to any published sequence. There are fewer than five copies of this transposable element present per genome in the fungus.     

Molecular Cloning, Genomic Organization, and Expression of a Testicular Isoform of Hormone-Sensitive Lipase

By catalyzing the rate-limiting step in adipose tissue lipolysis, hormone-sensitive lipase (HSL) is an important regulator of energy homeostasis. The role and importance of HSL in tissues other than adipose are poorly understood. We report here the cloning and expression of a testicular isoform, designated HSL_tes. Due to an addition of amino acids at the NH₂-termini, rat and human HSL_tesconsist of 1068 and 1076 amino acids, respectively, compared to the 768 and 775 amino acids, respectively, of the adipocyte isoform (HSL_adi). A novel exon of 1.2 kb, encoding the human testis-specific amino acids, was isolated and mapped to the HSL gene, 16 kb upstream of the exons encoding HSL_adi. The transcribed mRNA of 3.9 kb was specifically expressed in testis. No significant similarity with other known proteins was found for the testis-specific sequence. The amino acid composition differs from the HSL_adisequence, with a notable hydrophilic character and a high content of prolines and glutamines. COS cells, transfected by the 3.9-kb human testis cDNA, expressed a protein of the expected molecular mass (M_r≈ 120,000) that exhibited catalytic activity similar to that of HSL_adi. Immunocytochemistry localized HSL to elongating spermatids and spermatozoa; HSL was not detected in interstitial cells.     

Molecular evolution of mammalian lactate dehydrogenase-A genes and pseudogenes: association of a mouse processed pseudogene with a B1 repetitive sequence

A mouse genomic clone containing a lactate dehydrogenase-A (LDH-A) processed pseudogene and a B1 repetitive element was isolated, and a nucleotide sequence of approximately 3 kb was determined. The pseudogene and B1 element are flanked by perfect 13-bp repeats, and the B1 sequence starts at 14 nucleotides 3' to the presumptive polyadenylation signal of the pseudogene. The nucleotide sequences of the LDH-A genes and processed pseudogenes from mouse, rat, and human were compared, and a phylogenetic tree was constructed. The rate and pattern of nucleotide substitutions in the LDH-A pseudogenes are similar to previously reported results (Li et al. 1984). The average rate of nucleotide substitutions in the LDH-A pseudogenes is 4.3 X 10(- 9)/site/year. The substitutions of C----T and G----A are most frequent, and A----G substitutions are relatively high. The rate of synonymous substitutions in the LDH-A genes is 5.3 X 10(-9), which is not significantly higher than the average rate of 4.7 X 10(-9) for 35 mammalian genes. The rate of nonsynonymous substitutions in the LDH-A genes is 0.20 X 10(-9), which is considerably lower than the average rate of 0.88 X 10(-9) for 35 mammalian genes. Thus, the mammalian LDH-A gene appears to be highly conserved in evolution.      

3, 3′-diindolylmethane Enhances the Effectiveness of Herceptin against HER-2/Neu-Expressing Breast Cancer Cells

Herceptin failure is a major clinical problem in breast cancer. A subset of breast cancer patients with high HER-2/neu levels eventually experience metastatic disease progression when treated with Herceptin as a single agent. Mechanistic details of development of this aggressive disease are not clear. Therefore, there is a dire need to better understand the mechanisms by which drug resistance develops and to design new combined treatments that benefit patients with aggressive breast cancer and have minimal toxicity. We hypothesized that 3, 3′-diindolylmethane (DIM), a non-toxic agent can be combined with Herceptin to treat breast cancers with high levels of HER-2/neu. Here, we evaluated the effects of Herceptin alone and in combination with DIM on cell viability, apoptosis and clonogenic assays in SKBR3 (HER-2/neu-expressing) and MDA-MB-468 (HER-2/neu negative) breast cancer cells. We found that DIM could enhance the effectiveness of Herceptin by significantly reducing cell viability, which was associated with apoptosis-induction and significant inhibition of colony formation, compared with single agent treatment. These results were consistent with the down-regulation of Akt and NF-kB p65. Mechanistic investigations revealed a significant upregulation of miR-200 and reduction of FoxM1 expression in DIM and Herceptin-treated breast cancer cells. We, therefore, transfected cells with pre-miR-200 or silenced FoxM1 in these cells for understanding the molecular mechanism involved. These results provide experimental evidence, for the first time, that DIM plus Herceptin therapy could be translated to the clinic as a therapeutic modality to improve treatment outcome of patients with breast cancer, particularly for the patients whose tumors express high levels of HER-2/neu.     

Islands within an island: Repeated adaptive divergence in a single population

Physical barriers to gene flow were once viewed as prerequisites for adaptive evolutionary divergence. However, a growing body of theoretical and empirical work suggests that divergence can proceed within a single population. Here we document genetic structure and spatially replicated patterns of phenotypic divergence within a bird species endemic to 250 km² Santa Cruz Island, California, USA. Island scrub‐jays (Aphelocoma insularis) in three separate stands of pine habitat had longer, shallower bills than jays in oak habitat, a pattern that mirrors adaptive differences between allopatric populations of the species’ mainland congener. Variation in both bill measurements was heritable, and island scrub‐jays mated nonrandomly with respect to bill morphology. The population was not panmictic; instead, we found a continuous pattern of isolation by distance across the east–west axis of the island, as well as a subtle genetic discontinuity across the boundary between the largest pine stand and adjacent oak habitat. The ecological factors that appear to have facilitated adaptive differentiation at such a fine scale—environmental heterogeneity and localized dispersal—are ubiquitous in nature. These findings support recent arguments that microgeographic patterns of adaptive divergence may be more common than currently appreciated, even in mobile taxonomic groups like birds.     

Does Auxin Binding Protein 1 Control Both Cell Division and Cell Expansion?

The Auxin-Binding Protein 1 (ABP1) was identified over 30 years ago thanks to it''s high affinity for active auxins. ABP1 plays an essential role in plant life yet to this day, its function remains ‘enigmatic.’ A recent study by our laboratory shows that ABP1 is critical for regulation of the cell cycle, acting both in G₁ and at the G₂/M transition. We showed that ABP1 is likely to mediate the permissive auxin signal for entry into the cell cycle. These data were obtained by studying a conditional functional knock-out of ABP1 generated by cellular immunization in the model tobacco cell line, Bright Yellow 2.Key Words: auxin responses, auxin-binding protein 1, immunomodulation, cellular immunisation     

A Nomadic Subtelomeric Disease Resistance Gene Cluster in Common Bean

The B4 resistance (R) gene cluster is one of the largest clusters known in common bean (Phaseolus vulgaris [Pv]). It is located in a peculiar genomic environment in the subtelomeric region of the short arm of chromosome 4, adjacent to two heterochromatic blocks (knobs). We sequenced 650 kb spanning this locus and annotated 97 genes, 26 of which correspond to Coiled-Coil-Nucleotide-Binding-Site-Leucine-Rich-Repeat (CNL). Conserved microsynteny was observed between the Pv B4 locus and corresponding regions of Medicago truncatula and Lotus japonicus in chromosomes Mt6 and Lj2, respectively. The notable exception was the CNL sequences, which were completely absent in these regions. The origin of the Pv B4-CNL sequences was investigated through phylogenetic analysis, which reveals that, in the Pv genome, paralogous CNL genes are shared among nonhomologous chromosomes (4 and 11). Together, our results suggest that Pv B4-CNL was derived from CNL sequences from another cluster, the Co-2 cluster, through an ectopic recombination event. Integration of the soybean (Glycine max) genome data enables us to date more precisely this event and also to infer that a single CNL moved from the Co-2 to the B4 cluster. Moreover, we identified a new 528-bp satellite repeat, referred to as khipu, specific to the Phaseolus genus, present both between B4-CNL sequences and in the two knobs identified at the B4 R gene cluster. The khipu repeat is present on most chromosomal termini, indicating the existence of frequent ectopic recombination events in Pv subtelomeric regions. Our results highlight the importance of ectopic recombination in R gene evolution.In the human genome, extensive cytogenetic and sequence analyses have revealed that subtelomeres are hot spots of interchromosomal recombination and segmental duplications (Linardopoulou et al., 2005). This peculiar dynamic activity of subtelomeres has been reported in such diverse organisms as yeast and the malaria parasite Plasmodium (Louis, 1995; Freitas-Junior et al., 2000, 2005). As expected for a plastic region of the genome subject to reshuffling through recombination events, subtelomeres exhibit unusually high levels of within-species structural and nucleotide polymorphism (Mefford and Trask, 2002). In plants, this plasticity of subtelomeres has not been identified in Arabidopsis (Arabidopsis thaliana; Heacock et al., 2004; Kuo et al., 2006) and, to our knowledge, has not yet been investigated at a large scale for other plant species with full genome sequences available. Regarding Arabidopsis, the apparent lack of high subtelomeric recombination may reflect its small and simple subtelomeres, mirroring its small genome size and relative paucity of repetitive sequences (Heacock et al., 2004; Kuo et al., 2006).Repetitive sequences, such as satellite DNA and retroelements, constitute an important fraction of every eukaryotic genome and therefore constitute the environment in which genes are expressed. Satellite DNA can be defined as highly reiterated noncoding DNA sequences, organized as long arrays of head-to-tail linked repeats of 150- to 180-bp or 300- to 360-bp monomers located in the constitutive heterochromatin (Plohl et al., 2008). Despite their ubiquity in eukaryotic genomes, little is known about the mechanisms that allow these elements to accumulate. Early hypotheses considered them to be nonfunctional “selfish” or “junk” DNA segments that increase or decrease their frequency without any advantage or disadvantage for an organism (Ohno, 1972; Orgel and Crick, 1980). However, identification of satellite DNA at structurally important parts of chromosomes, such as centromeres, has suggested functional roles of satellite DNA (Ma and Jackson, 2006; Kawabe and Charlesworth, 2007). Satellite DNA can also be localized in knobs, which are cytologically visible regions of highly condensed chromatin (heterochromatin) that are distinct from pericentromeric regions in pachytene chromosomes (Fransz et al., 2000; Gaut et al., 2007; Lamb et al., 2007).The survival of most organisms depends on the presence of specific genetic systems that maintain diversity in order to respond to changing environments. Plants, like animals, are continually challenged by a large array of pathogens. To perceive and counter pathogen attack, plants have evolved disease resistance (R) genes. The largest class of R genes encodes proteins containing a central Nucleotide-Binding Site (NBS) domain, a C-terminal Leucine-Rich Repeat (LRR) domain, and a variable N-terminal domain. These R proteins detect the presence of disease-causing bacteria, oomycetes, fungi, nematodes, insects, and viruses by sensing either specific pathogen effector molecules produced during the infection process or key molecules in the plant cell that may be attacked by pathogen effectors (Dangl and McDowell, 2006). The evolution of new R genes serves to counteract the evolution of novel virulence factors from the pathogens (McDowell and Simon, 2008). Among this prevalent class of R gene, two subclasses, corresponding to two ancient lineages (Bai et al., 2002; Meyers et al., 2003; Ameline-Torregrosa et al., 2008), have been identified based on the N-terminal domain of the R protein: the Coiled-Coil (CC)-NBS-LRR (CNL) and the Toll-Interleukin receptor (TIR)-NBS-LRR (TNL). Genome studies have demonstrated that NBS-LRR (NL) sequences are abundant in any plant genome. For example, annotation of the Arabidopsis, rice (Oryza sativa), poplar (Populus trichocarpa), Medicago truncatula (Mt), grape (Vitis vinifera), Lotus japonicus (Lj), and papaya (Carica papaya) genomes identified at least 149, 480, 317, 333, 233, 229, and 55 genes encoding NL proteins, respectively (Bai et al., 2002; Meyers et al., 2003; Zhou et al., 2004; Tuskan et al., 2006; Velasco et al., 2007; Ameline-Torregrosa et al., 2008; Kohler et al., 2008; Ming et al., 2008; Sato et al., 2008). NL sequences are often located at complex loci (Smith et al., 2004), as exemplified by Arabidopsis, where two-thirds of them are organized in tightly linked clusters (Meyers et al., 2003; Leister, 2004; McDowell and Simon, 2006). Evolution of NL sequences in the Arabidopsis genome has been investigated according to their phylogenetic positions and physical locations. Although tandem duplications explain the origin of a large fraction of NLs, it seems that ectopic recombination has also played a role in Arabidopsis NL evolution, since mixed clusters comprising evolutionarily distant NL exist. Ectopic recombination is also evident when phylogenetically close R genes are physically dispersed on different chromosomes (Leister, 2004; McDowell and Simon, 2006). These results confirm pioneer macrosynteny studies between related monocot species suggesting the existence of NL movement in plant genomes. Indeed, extensive loss of collinearity between NL sequences between rice and barley (Hordeum vulgare), which diverged 50 million years ago (Mya), has suggested rapid reorganization of NL sequences (Leister et al., 1998; Leister, 2004). However, our knowledge of the molecular evolution of R genes remains limited due to the still small number of complete plant genome sequences available to date. Detailed comparative study across taxa at different evolutionary distances is needed to see how R gene clusters evolve at various time scales.Legumes (Fabaceae) constitute the third largest family of flowering plants and represent the second most important family of agronomically important plants after Poaceae (Graham and Vance, 2003). As a result of recent sequencing efforts, legumes are one of the few plant families with extensive genome sequences in different species, since the soybean (Glycine max [Gm]) genome sequence is complete (http://www.phytozome.net/soybean.php) and both Mt and Lj genome sequences are nearly complete (Young et al., 2005; Sato et al., 2008). Consequently, the legume family is extremely well adapted for comparative phylogenomic approaches, in which phylogenetic inference is combined with structural genomic analyses (Ammiraju et al., 2008). Common bean (Phaseolus vulgaris [Pv]) is the most important grain legume for direct human consumption (Broughton et al., 2003). Pv is a selfing species and has a small diploid genome (2n = 22) of 588 Mb (Bennett and Leitch, 1995). Conservation of genome macrostructure (macrosynteny) has been reported between several legumes, including common bean and the two model legume species Mt and Lj genomes (Zhu et al., 2005; Hougaard et al., 2008). However, the extent of gene order conservation at the DNA sequence level has not yet been evaluated within orthologous chromosome segments between Pv and the two model legume species.In the genome of common bean, many disease R genes are clustered at complex loci located at the ends (rather than the centers) of linkage groups (LGs; Vallejos et al., 2006; Geffroy et al., 2008). For example, Colletotrichum lindemuthianum Co-2 R specificity maps at one end of LG B11 (Adam-Blondon et al., 1994). Molecular analysis has revealed that this locus consists of a tandem array of CNL sequences (Geffroy et al., 1998; Creusot et al., 1999). Another CNL-rich region has been identified at the end of LG B4 in the vicinity of R specificities and R quantitative trait loci against a large selection of pathogens, including C. lindemuthianum, Uromyces appendiculatus, and the bacterium Pseudomonas syringae (Geffroy et al., 1998, 1999; Miklas et al., 2006). Recently, fluorescence in situ hybridization (FISH) analysis revealed that this complex R cluster is located in the subtelomeric region of the short arm of chromosome 4 and includes two knobs (Geffroy et al., 2009). In a sequencing effort focused on CNL sequences, we have previously identified 17 CNL sequences of the B4 locus (referred to as B4-CNL) from Pv genotype BAT93 (Ferrier Cana et al., 2003, 2005; Geffroy et al., 2009). In the BAT93 genotype, these B4-CNL sequences are located on both sides of the subterminal knob (Geffroy et al., 2009).To investigate the organization and the evolutionary origin of the subtelomeric B4 R gene cluster, we have sequenced approximately 650 kb of the Pv B4 R gene cluster, revealing that, in genotype BAT93, CNL are spread out in four subclusters, separated by non-CNL-encoding genes. This Pv sequence was then compared gene by gene with the sequenced portions of the three sequenced legume genomes, Mt, Lj, and Gm. Conserved microsynteny (conservation of local gene repertoire, order, and orientation) was observed, except for the CNL sequences, which appear to be completely absent in the corresponding regions of Mt and Lj. In this study, by combining genomics, phylogenetic, and cytogenetic approaches, we provide evidence that ectopic recombination in subtelomeric regions between nonhomologous chromosomes (4 and 11), involving a single CNL, gave rise to the Pv B4 R gene cluster. Chromosomal distribution of a new satellite DNA tandem repeat, referred to as khipu, suggests that ectopic recombination events in subtelomeric regions of bean nonhomologous chromosomes are frequent. Our results highlight the importance of ectopic recombination as an important evolutionary mechanism for the evolution of disease resistance genes.     

Breeding latitude and timing of spring migration in songbirds crossing the Gulf of Mexico

Each spring, millions of songbirds migrate across the Gulf of Mexico on their way to breeding sites in North America. Data from radar and migration monitoring stations have revealed broad patterns in the spatial and temporal course of trans-Gulf migration. Unfortunately, we have limited information on where these birds have previously spent the winter and where they are migrating to breed. Here we measure stable-hydrogen isotopes in feathers (δD_f) to infer the breeding latitude of five species of songbirds – hooded warblers Wilsonia citrina , American redstarts Setophaga ruticilla , black-and-white warblers Mniotilta varia , ovenbirds Seiurus aurocapilla , and northern waterthrushes S. noveboracensis – that were captured at a stopover site along the coast of southwestern Louisiana in spring 2004. Values of δD_f across all species ranged from −163 to −35‰ (n=212), and within most species the range was consistent with the latitudinal extent of known breeding sites in central and eastern North America. Individuals that arrived first along the northern Gulf coast had δD_f values indicative of southerly breeding sites in hooded warblers, American redstarts, black-and-white warblers, and ovenbirds, but no relationship was found between passage timing and δD_f for northern waterthrushes. Our findings suggest that spring passage is often timed to coincide with the emergence of suitable conditions on breeding areas, with southern breeding birds migrating first.