Scanning electron microscopy of post-ejaculatory spermiogenesis in the tick Ornithodoros moubata

The final stages of spermiogenesis in ticks occur in the female genital tract. Scanning electron microscopy was used to follow the morphologic changes that occur in the sperm during this post-ejaculatory spermiogenesis in the African soft tick, Ornithodoros moubata, and to determine a time sequence for its occurrence in vivo. Characteristic features of the maturing and mature cell described include (1) differentiation and detachment of the operculum, (2) changes in cell shape corresponding to different developmental stages, (3) passive migration of the nucleus and acrosome from an anterior to a posterior position, and (4) eversion of that portion of the acrosomal canal containing the nucleus and acrosome. A possible fate for the remainder of the acrosomal canal is suggested by extrusion and detachment of spherical structures, the ‘posterior bubbles’, from the posterior end of the mature supermatozoon. A mechanism for cellular elongation resulting from contractions of the outer sheath is proposed.     

长角血蜱卵黄蛋白的纯化及其性质

用凝胶过滤与离子交换层析、蛋白质电泳和糖脂蛋白染色等方法提取纯化长角血蜱Haemaphysalis longicornis卵黄蛋白,并对其性质进行了研究。PAGE和SDS-PAGE分析表明,长角血蜱的卵黄蛋白只有一种,由8个亚基组成,亚基的相对分子质量分别为112 kD, 103 kD, 80 kD, 78 kD, 71 kD, 68 kD, 62 kD和52 kD,卵黄蛋白经苏丹黑B和希夫试剂染色呈阳性,表明是一种含血红素的糖脂蛋白。     

Purification of insect vitellogenin and vitellin by gel-immobilized ferric chelate.

Vitellogenin and vitellin of Manduca sexta and some other insect species were purified by immobilized metal ion affinity chromatography. Ferric ion was chosen as the immobilized metal ion. Agarose-bound carboxymethylpicolylamine was used as the chelating adsorbent for the ferric ion. Vitellogenin and vitellin, both phosphorylated lipoproteins, were shown to bind specifically to the iron. The general applicability of immobilized ferric ion affinity chromatography for the purification of insect vitellogenin and vitellin is suggested.     

Purification and partial characterization of vitellin from the eggs of the hard tick,Dermacentor variabilis

The major yolk proteins were purified from the eggs of the hard tick, Dermacentor variabilis using gel filtration and ion exchange chromatography. Two vitellin proteins were identified and designated vitellin A (480 kilodaltons; kDa) and vitellin B (370 kDa). The isolectric points were pH 6.1 and 6.25, respectively. The absorption maxima for both proteins were 280 and 400 nm. The buoyant density of vitellin A was 1.281 g/ml and vitellin B 1.278 g/ml. The vitellins were hemoglycolipoproteins as indicated by selective staining of polyacrylamide gels, carbohydrate analyses and lipid analyses. Under reducing conditions (SDS-PAGE), vitellin A had eight major polypeptides at 135, 110, 98, 80, 67, 50, 45, and 35 kDa. Vitellin B was identical to vitellin A with the addition of a 93 kDa subunit. The only carbohydrate detectable in the proteins was mannose. The neutral lipids detected in both proteins were cholesteryl esters, triglycerides, free fatty acids and their methyl esters, and cholestrol. The only detectable phospholipid in both proteins was phosphatidylethanolamine. The purified vitellins were immunologically identical to female hemolymph proteins but not to host hemoglobin. Antivitellin antibodies to vitellin were used to identify possible locations of vitellogenin in the organs of ovipositing females.     

Purification and molecular properties of vitellin from the silkworm,Bombyx mori

Vitellin was purified from the eggs of the silkworm, Bombyx mori by a simple method which included a specific precipitation at pH 6 under low ionic concentration and DEAE-cellulose column chromatography. The final preparation was highly homogeneous as judged by gel electrophoresis, electron microscopy and ultracentrifugation.Vitellin was defined as glycolipoprotein with a sedimentation coefficient (S_{20, W}) of 13.5S and a molecular weight of 440,000. The molecule was almost spherical in shape with a diameter of 13 nm. The molecule contained 3% mannose and 7.5% total lipids which comprised triacylglycerol, diacylglycerol, cholesterol, phosphatidylcholine and phosphatidylethanolamine. The amino acid composition displayed a high content of glutamic and aspartic acids and a low content of methionine. The molecule was composed of two non-identical subunits with molecular weights of 180,000 and 42,000, and the native molecule was assumed to be a tetramer composed of two molecules of each of these subunits. Separation of the two subunits was achieved, and mannose was covalently associated only with the heavier subunit.The rabbit anti-egg vitellin antibody cross-reacted with the haemolymph vitellogenin but not with other haemolymph proteins, nor with the vitellogenin from Locusta migratoria. The antibody also reacted with the haemolymph vitellogenin of the silkworm, Philosamia cynthia.     

Studies on the application of the sterility method in the tick Ornithodoros tholozani

A method for the application of sterile male technique in Ornithodoros tholozani is described and its practicality is discussed.Techniques for rearing large numbers on rats, and feeding through artificial membranes are given.Nymphs are prevented from molting at doses of 2000r and above if applied before feeding. Both sexes emerging from nymphs irradiated by more than 2000r, two weeks after feeding, are sterile. These males are not competitive due to lack of sperm.Females become sterile after irradiation by more than 2000r, whereas males require 16000r in order to induce 99% dominant lethality. These males proved to be effective in competing with normal males.

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Études sur l'application à la tique, Ornithodoros Tholozani, de la méthode de stérilisation

Résumé La tique O. tholozani, qui est le vecteur de la fièvre recurrente humaine, se trouve en tant que populations isolées, généralement dans des cavernes dans tout le Proceh Orient. Les tiques rampent profondément dans le sol et résistent plusieurs années à l'inanition.On a développé une méthode de lutte contre cette tique par l'inondation de l'habitat avec des mâles stériles.L'élevage en masse des tiques a été effectué en les nourrissant sur rats à un intervalle de deux mois, ou en les nourrissant de sang de buf défibriné sur des membranes artificielles.Les tiques ont été stérilisées en les irradiant avec une source Co⁶⁰ émettant 7700r/min. Les nymphes irradiées avec 2000 r et plus n'ont pas mué si elles ont été irradiées avant d'avoir reçu la nourriture. Si elles ont été irradiées deux semaines après avoir reçu la nourriture, les adultes formés sont devenus stériles. Les mâles obtenus des nymphes traitées ne contenaient pas de sperme, et à cause de cela, n'ont pas été des concurrents des mâles normaux.Les femelles adultes irradiées avec 2000r sont devenues stériles. Les mâles adultes nécessitent 16000r pour causer 99% de léthalité dominante dans le sperme. Ces mâles ont prouvé être effectifs en compétition avec les mâles normaux, pour une période suffisamment longue. Pendant cette période les mâles n'ont pas recouvré leur fertilité.L'alimentation sur sang immédiatement après l'irradiation n'a pas affecté les mâles, mais seulement quelques tiques ainsi traitées ont pris difficilement une seconde nourriture.A cause de cela, on fît un plan de nourrir les tiques sur membranes, après irradiation et avant d'être lâchées.

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This investigation was supported by a grant from the Ford Foundation.     

Cutaneous and systemic cellular responses induced by the feeding of the argasid tick Ornithodoros parkeri

Carolyn M. Johnston and Stephen J. Brown 1985. Cutaneous and systemic cellular responses induced by the feeding of the argasid tick Ornithodoros parkeri. International Journal for Parasitology15: 621–628. Initial feeding by Ornithodoros parkeri ticks induced a significant blood basophilia in guinea pigs, with a minimal cutaneous basophil response. Hosts challenged 14 days later, however, exhibited significantly depressed blood basophil levels associated with a marked accumulation of these cells at tick feeding sites in the tissue. Blood eosinophil levels in primary and secondary hosts were comparable, but eosinophil levels at tick feeding sites in challenged animals were significantly greater than levels in primary hosts. Furthermore, challenge tick feeding resulted in the activation of primary tick feeding sites on the opposite flank that became erythematous 90 min after challenge and indurated within 24 h. Histologically, these activated primary feeding sites 90 min after challenge on the opposite flank were marked by a dominant eosinophil response (314 ± 128 cells, 59% of the infiltrate) with a marked basophil component (145 ± 67 cells, 28% of the infiltrate) that resembled the active challenge feeding sites 24 h after infestation (24 ± 52 cells, 76% of the infiltrate); 90 min after challenge active feeding sites had a weak basophil response (2 ± 1 cells) similar to uninfested controls. These results suggest the chronic nature of tick bites with an apparent continual recruitment of basophils that is probably a result of slow antigen release over time by appropriately sensitized antigen presenting cells. Primary tick feeding sites in guinea pigs previously exposed to Xenopsylla cheopis fleas, on the opposite flank, contained a marked eosinophilia (63 ± 25 cells) compared to primary tick feeding sites in naive guinea pigs (2 ± 0 cells); suggesting the possibility of cross reactivity between flea and tick antigens     

Biosynthesis,purification, and characterization of Aedes aegypti vitellin and vitellogenin

Vitellin, the major egg yolk protein, and vitellogenin, the hemolymph precursor of egg yolk protein, have been purified to apparent homogeneity from the mosquito Aedes aegypti. The purification procedure included chromatography on ion exchange, hydrophobic, and gel filtration columns. Vitellin and vitellogenin have a similar molecular weight (M_r 300,000) on gel filtration columns. However, the molecular weights of vitellin and vitellogenin, as determined from SDS electrophoresis, were 393,000 and 337,000, respectively. Vitellin in sodium dodecyl sulfate released six subunits of molecular weight 116,000, 83,000, 75,000, 54,000, 36,000, and 29,000, whereas vitellogenin released only three subunits (155,000, 120,000, and 62,000). The average molecular weights of vitellin and vitellogenin after gel filtration and SDS electrophoresis were 346,000 and 318,000, respectively. Vitellin has a high content of aspartic acid and glutamic acid, and a low content of histidine, methionine, cysteine, and tryptophan. Vitellin also contains 0.9% mol of glucosamine and no galactosamine. The isoelectric points of vitellin and vitellogenin are at pH 6.4 and 6.3, respectively. Aedes aegypti fat bodies incubated for short intervals in tissue culture medium in the presence of [³H]valine showed incorporation by radio-immunoprecipitation and SDS electrophoresis into three primary vitellogenin polypeptides of molecular weights (± SEM) 156,000 ± 4,000, 114,000 ± 5,000, and 62,000 ± 400 inside the fat body and 162,000 ± 3,000, 118,200 ± 2,000, and 63,000 ± 300 in the medium. These results suggest that the molecular weight of vitellogenin synthesized inside the fat body (M_r 332,000) remains unchanged when secreted into the hemolymph (M_r 343,000). The three vitellogenin subunits are processed by the ovary into six subunits which are then deposited in the yolk granules as vitellin.     

Binding and storage of heme by vitellin from the cattle tick,Boophilus microplus

We have previously shown (, Curr. Biol. 9, 703-706) that the cattle tick Boophilus microplus does not synthesize heme, relying solely on the recovery of the heme from the diet to make all its hemeproteins. Here we present evidence that Vitellin (VN(1)), the main tick yolk protein, is a reservoir of heme for embryo development. VN was isolated from eggs at different days throughout embryogenesis. Immediately after oviposition, Boophilus VN contains approximately one mol of heme/mol of protein. During embryo development about one third of egg VN is degraded. The remaining VN molecules bind part of the heme released. These results suggest that VN functions as a heme reservoir, binding any free heme that exceeds the amount needed for development. In vitro measurement of the binding of heme to VN showed that each VN molecule binds up to 31 heme molecules. The association of heme with VN strongly inhibits heme-induced lipid peroxidation, suggesting that binding of heme is an important antioxidant mechanism to protect embryo cells from oxidative damage. This mechanism allows this hematophagous arthropod to safely store heme obtained from a blood meal inside their eggs for future use. Taken together our data suggest that, besides its known roles, VN also plays additional functions as a heme deposit and an antioxidant protective molecule.     

Synthesis and organization of vitellogenin and vitellin molecules from the land crab Potamon potamios

We have previously reported that vitellogenin (Vg) of some female animals contained four polypeptides with molecular mass of 181, 115, 105 and 85 kDa, whereas Vg of most animals contained three polypeptides with molecular mass of 115, 105 and 85 kDa. In the present investigation, we examined whether the 181 kDa polypeptide is the precursor of 115 and 105 kDa Vg and vitellin (Vn) polypeptides. Labeling studies, using [35S]methionine on normal vitellogenic animals, showed that the radioactivity was distributed first among the 181 and 85 kDa polypeptides. SDS-PAGE analysis of purified hemolymph Vg from eyestalk ablated female animals revealed in most animals two polypeptides with an apparent molecular mass of 181 and 85 kDa. These results from in vivo experiments corroborated the view that the 115 and 105 kDa Vg and Vn polypeptides are derived from heaviest 181 kDa polypeptide. In addition it was demonstrated that hepatopancreas and ovary of Potamon potamios incubated in vitro with [35S]methionine synthesized five polypeptides with apparent molecular mass of 224, 181, 115, 105, and 85 kDa while the hepatopancreas appeared to secrete the 181, 115, 105 and 85 kDa polypeptides. The major 115, 105 and 85 kDa polypeptides were found to be components of egg Vn, while the 224 kDa polypeptide was found to be minor component of Vg and Vn from hepatopancreas and ovary extracts, respectively. We conclude that the Vn polypeptides produced by ovary are similar to those produced by hepatopancreas.     

Purification and properties of methanol dehydrogenase from Methylophaga marina

Purification of methanol dehydrogenase from Methylophaga marina, in order to avoid the instability observed in crude extracts, was achieved initially by a rapid procedure using mainly an aqueous two-phase partition system composed of polyethylene glycol 1000 (50%, v/v) and potassium phosphate (50%, w/v). The purified enzyme gave a single band of protein after SDS-polyacrylamide gel electrophoresis. Antiserum raised against purified methanol dehydrogenase was used to detect possible protein contaminants in the enzyme preparation. The enzyme is an NAD-independent dehydrogenase containing pyrrolquinoline quinone (PQQ) as a prosthetic group. It is made of two apparently identical subunits giving a total MW of 145,000 for the native enzyme. The isoelectric point is 6.4. In addition to methanol and formaldehyde, multicarbon primary alcohols and aldehydes as well as secondary alcohols can be used as substrates. Except for ammonium chloride, which is a necessary activator in vitro, no effector was found which could modify the rate of enzyme activity under standard conditions of the assay. Although the main properties of this methanol dehydrogenase are similar to those already described in the literature, it does not belong in any of the five categories described by Anthony.     

Purification and properties of a Mg-dependent ATPase from chloroplasts of Euglena gracilis

Isolated chloroplasts of Euglena gracilis contain highly active ATPases. The ATPase activity in the chloroplasts is usually much higher than the maximal rate of photophosphorylation obtainable and is due to a number of different enzymes.

One of these ATPases, Mg²⁺-dependent and with a low pH optimum, has been solubilized with the aid of detergents and purified approx. 20-fold. The optimal activity of the enzyme is at pH 5.5, and the optimal Mg²⁺ concentration is 5·10⁻³ M. The enzyme hydrolyzes dATP more rapidly than ATP, although the K_m for both substrates is the same. Other nucleotide triphosphates are hydrolyzed very slowly while ADP or pyrophosphate are not hydrolyzed at all. Oligomycin, carbonylcyanide m-chlorophenylhydrazone, and ADP inhibit the enzyme, the latter competitively.

The level of the enzyme is highest in chloroplasts from rapidly dividing cells, and reaches a minimum in chloroplasts from maturing cultures which have attained their maximal photosynthetic activity. It is postulated that the enzyme has a role in controlling chloroplast development.     

Purification and properties of a chitinase from Penicillium sp. LYG 0704

The chitinase producing Penicillium sp. LYG 0704 was procured from soil of the Chonnam National University crop field. The chitinase activity was detected after the first day which increased gradually and reached its maximum after 3 days of cultivation. The chitinase was purified from a culture medium by precipitation with isopropanol and column chromatography with Mono Q and Butyl-Sepharose. The molecular mass of chitinase was estimated to be 47 kDa by SDS–PAGE. Optimal pH and temperature were 5.0 and 40 °C, respectively. The N-terminal amino acid sequence of the enzyme was determined to be ¹AGSYRSVAYFVDWAI¹⁵. The fully cloned gene, 1287 bp in size, encoded a single peptide of 429 amino acids. BLAST search of the chitinase gene sequence showed similarity with chitinase of Aspergillus fumigatus Af293 chitinase gene (58%) and A. fumigatus class V chitinase ChiB1 gene (56%).     

Purification and some properties of a carboxypeptidase B from dogfish Scyliorhinus canicula

A carboxypeptidase B (CPB) has been purified from dogfish (Scyliorhinus canicula) pancreas and partially characterized. The purification procedure included acetone precipitation, ion-exchange chromatography on a CM-cellulose column and gel filtration on Sephadex G-75. The purified enzyme migrates as a single band both on PAGE and SDS-PAGE. Its molecular mass is estimated to be about 32 kDa. The optimum of activity is obtained at pH 7.5–8.2. The enzyme is inhibited by typical metal-chelating agents (EDTA and o-phenanthroline) and by Hg²⁺. It is activated by Co²⁺, l-cysteine and by heat treatment at 40° and 50°C. Kinetic parameters, K_m and k_cat, of native enzyme, Co²⁺-activated CPB and heat-treated CPB have been determined     

Purification and properties of two exo-cellobiohydrolases from a cellulolytic culture of Fusarium lini

Two distinct exo-cellobiohydrolases (1,4-β-d-glucan cellobiohydrolase, EC 3.2.1.91) have been isolated from culture filtrates of Fusarium lini by repeated ammonium sulphate fractionation and isoelectric focusing. The purified enzymes were evaluated for physical properties, kinetics and the mechanism of their action. The results of this work were as follows. (1) A two-step enzyme purification procedure was developed, involving isoelectric focusing and ammonium sulphate fractionation. (2) Yields of pure cellobiohydrolases I and II were 45 and 36 mg l^?1 of culture broth, respectively. (3) Both enzymes were found to be homogeneous, as determined by ultracentrifugation, isoelectric focusing, electrophoresis in polyacrylamide gels containing SDS and chromatography on Sephadex. (4) The molecular weights of the two cellobiohydrolases, as determined by gel filtration and SDS gel electrophoresis, were 50 000–57 000. (5) Both cellobiohydrolases had low viscosity-reducing and reducing sugar activity from carboxymethyl cellulose and high activity with Walseth cellulose and Avicel. (6) The enzymes produced only cellobiose as the end product from filter paper and Avicel, indicating that they are true cellobiohydrolases. (7) Cellobiohydrolase I hydrolysed d-xylan whereas cellobiohydrolase II was inactive towards d-xylan. (8) There was a striking synergism in filter paper activity when cellobiohydrolase was supplemented with endo-1,4-β-d-glucanase [cellulase, 1,4-(1,3;1,4)-β-d-glucan 4-glucanohydrolase, EC 3.2.1.4] and β-d-glucosidase (β-d-glucoside glucohydrolase, EC 3.2.1.21).