Host plants of the tarnished plant bug (Heteroptera: Miridae) in Central Texas

The tarnished plant bug, Lygus lineolaris (Palisot de Beauvois), has taken on added importance as a pest of cotton in the Cotton Belt after successful eradication efforts for the boll weevil (Anthonomus grandis grandis Boheman). Because the Southern Blacklands region of Central Texas is in advanced stages of boll weevil eradication, blooming weeds and selected row crops were sampled during a 3-yr study to determine lygus species composition and associated temporal host plants. L. lineolaris was the sole lygus species in the region. Thirteen previously unreported host plants were identified for L. lineolaris, of which 69% supported reproduction. Rapistrum rugosum L. Allioni and Ratibida columnifera (Nuttall) Wooton and Standley were primary weed hosts during the early season (17 March to 31 May). Conyza canadensis L. Cronquist variety canadensis and Ambrosia trifida L. were primary weed hosts during the midseason (1 June to 14 August) and late-season (15 August to 30 November), respectively. Sisymbrium irio L. and Lamium amplexicaule L. sustained L. lineolaris populations during the overwintering period (1 December to 16 March). The proportion of females and numbers of nymphs found in R. rugosum, C. canadensis, A. trifida, and S. irio suggests these weeds supported reproductive adults during the early, mid-, and late season and overwintering period, respectively. Medicago sativa L. was the leading crop host for L. lineolaris; Glycine max L. Merrill did not yield L. lineolaris. Few L. lineolaris were collected in Gossypium hirsutum L. These results provide a more comprehensive assessment of host plants contributing to L. lineolaris populations in central Texas.     

The Association of the Vanin-1 N131S Variant with Blood Pressure Is Mediated by Endoplasmic Reticulum-Associated Degradation and Loss of Function

High blood pressure (BP) is the most common cardiovascular risk factor worldwide and a major contributor to heart disease and stroke. We previously discovered a BP-associated missense SNP (single nucleotide polymorphism)–rs2272996–in the gene encoding vanin-1, a glycosylphosphatidylinositol (GPI)-anchored membrane pantetheinase. In the present study, we first replicated the association of rs2272996 and BP traits with a total sample size of nearly 30,000 individuals from the Continental Origins and Genetic Epidemiology Network (COGENT) of African Americans (P = 0.01). This association was further validated using patient plasma samples; we observed that the N131S mutation is associated with significantly lower plasma vanin-1 protein levels. We observed that the N131S vanin-1 is subjected to rapid endoplasmic reticulum-associated degradation (ERAD) as the underlying mechanism for its reduction. Using HEK293 cells stably expressing vanin-1 variants, we showed that N131S vanin-1 was degraded significantly faster than wild type (WT) vanin-1. Consequently, there were only minimal quantities of variant vanin-1 present on the plasma membrane and greatly reduced pantetheinase activity. Application of MG-132, a proteasome inhibitor, resulted in accumulation of ubiquitinated variant protein. A further experiment demonstrated that atenolol and diltiazem, two current drugs for treating hypertension, reduce the vanin-1 protein level. Our study provides strong biological evidence for the association of the identified SNP with BP and suggests that vanin-1 misfolding and degradation are the underlying molecular mechanism.     

Ultrastructural localization of amiloride-sensitive sodium channels and Na+,K(+)-ATPase in the rat's olfactory epithelial surface

Several studies have indicated that olfactory responses are impeded by amiloride. Therefore, it was of interest to see whether, and if so which, olfactory epithelial cellular compartments have amiloride- sensitive structures. Using ultrastructural methods that involved rapid freezing, freeze-substitution and low temperature embedding of olfactory epithelia, this study shows that, in the rat, this tissue is immunoreactive to antibodies against amiloride sensitive Na(+)- channels. However, microvilli of olfactory supporting cells, as opposed to receptor cilia, contained most of the immunoreactive sites. Apices from which the microvilli sprout and receptor cell dendritic knobs had much less if any of the amiloride-antibody binding sites. Using a direct ligand-binding cytochemical method, this study also confirms earlier ones that showed that olfactory receptor cell cilia have Na+, K(+)-ATPase. It is proposed that supporting cell microvilli and the receptor cilia themselves have mechanisms, different but likely complementary, that participate in regulating the salt concentration around the receptor cell cilia. In this way, both structures help to provide the ambient mucous environment for receptor cells to function properly. This regulation of the salt concentration of an ambient fluid environment is a function that the olfactory epithelium shares with cells of transporting epithelia, such as those of kidney.      

Rapid low molecular weight polyethylene glycol embedding protocol for immunocytochemistry

We describe an alternative polyethylene glycol (PEG) embedding procedure which utilizes PEG 200 for dehydration and PEG 600 for infiltration and embedding of perfusion-fixed rat liver. PEG 600 has a melting point of 22 degrees C, enabling infiltration of fixed tissue to be performed at room temperature. Sections (2 microM) cut in a cryostat at -20 degrees C and immobilized in agarose were readily labeled by immunoperoxidase protocols with monoclonal antibodies to hepatocyte membrane antigens. Subsequent examination by light microscopy or by electron microscopy after re-embedding in resin and ultra-thin sectioning showed excellent preservation of morphology, with minimal impairment of antigenicity.     

Investigations into the efficacy of 1,N6-ethenoadenosine triphosphate as a substrate for contractility studies

1,N⁶-Ethenoadenosine triphosphate was found to support superprecipitation of actomyosin and contraction of fibers. Its reactivity toward myosin parallels that of ITP. The relevance of these results in elucidating the mechanism for myosin nucleotide triphosphatase is discussed.     

Structural changes in profilin accompany its binding to phosphatidylinositol, 4,5-bisphosphate.

The effect on the structure of profilin of phosphatidylinositol 4,5-bisphosphate (PIP2) binding was probed by fluorescence and circular dichroism (CD) spectroscopy. Fluorescence of Trp3 and Trp31 of profilin at 292 nm showed a linear decrease in solution emission at 340 nm as PIP2/profilin was increased from 0 to 80:1, apparently due to a static quenching mechanism involving formation of a nonfluorescent PIP2/profilin complex. CD spectra revealed an increase of up to 3.3-fold in the molar ellpticity at 222 nm for profilin as it binds PIP2, as well as changes in the Cotton effect between 250 and 310 nm. These results are consistent with a possible increase in the alpha-helix content of profilin triggered by the binding of PIP2.     

Inhibition of mammalian succinate dehydrogenase by carboxins.

Carboxin (5,6-dihydro-2-methyl-1,4-oxathiin-3-carboxanilide), a systemic fungicide, is known to inhibit the oxidation of succinate selectively in a variety of fungi and bacteria. Except for one report, the action of carboxin and of structurally related oxathiin derivatives on mammalian succinate dehydrogenase have not been investigated, however. In the present study, the inhibition of succinate oxidation by a number of carboxin derivatives have been studied using inner membrane preparations, purified particulate preparations (Complex II), and soluble preparations from beef heart. The site of action of carboxins has been studied by using a variety of electron acceptors. It has been concluded that carboxins inhibit mammalian succinate dehydrogenase by reacting at the same site as thenoyltrifluoroacetone but are effective at far lower concentrations. The maximal extent of inhibition by carboxins varies with the type of catalytic assay used and, in general, parallels the extent of inactivation brought about by cyanide, as if both types of agents modified the environment of an iron-sulfur component in the enzyme, presumably the superoxidized (HiPIP) Fe-S cluster.