刀豆氨酸对亚洲玉米螟生长发育的影响

以不同浓度刀豆氨酸注射和饲喂亚洲玉米螟`Ostrinia furnacalis`` 5龄幼虫,影响其以后各虫态的生长发育,有引起畸蛹和畸蛾的明显作用,发育成的雌蛾性腺发育受到抑制,卵管变短,卵细胞数减少。不同交配实验表明对发育成的雄蛾影响更为严重,能使其不育。供试幼虫48小时后取血样,表明血淋巴蛋白质区带与对照组不同,认为刀豆氨酸对亚洲玉米螟的上述作用可能与刀豆氨酸取代精氨酸参入蛋白质的结果有关。     

褐飞虱体内类酵母共生菌与氨基酸营养的关系

利用全纯人工饲料饲喂技术,研究了缺失不同氨基酸对高温(35℃)处理后的缺菌褐飞虱Nilaparvata lugens Stål相对生长速度、体内共生菌数量的影响,发现10种必需氨基酸对缺菌褐飞虱生长的影响明显大于10种非必需氨基酸,饲料中必需氨基酸的缺少对褐飞虱（特别是高温处理褐飞虱）体内共生菌数量有一定的刺激作用。分析了缺菌试虫体内氨基酸组成和转氨酶活性的变化规律,发现在摄取的氨基酸营养相同的条件下（用全纯饲料D-97饲养）,高温处理试虫体内蛋白质氨基酸组成无明显变化,而游离氨基酸总量明显上升,且必需氨基酸所占比例显著下降,其中组氨酸（His）、异亮氨酸（Ile）、亮氨酸（Leu）、赖氨酸（Lys）、蛋氨酸（Met）和苯丙氨酸（Phe）摩尔百分含量均显著下降,表明必需氨基酸的相对缺乏可能是体内蛋白质合成受阻的一个重要原因,推测这可能是由于试虫体内共生菌数减少致使所合成的必需氨基酸减少而引起。处理试虫体内谷氨酰胺合成酶（GS）和丙氨酸氨基转移酶（ALT）活性明显提高,天冬氨酸氨基转移酶(AST)活性显著降低,结合游离氨基酸中谷氨酰胺（Gln）显著增多,推测类酵母共生菌可能利用谷氨酰胺等为原料进行必需氨基酸的合成。     

感染球孢白僵菌后红火蚁体内蛋白质含量的变化

为了解球孢白僵菌Beauveria bassiana成功感染红火蚁Solenopsis invicta的生理生化机制, 本研究在室内条件下测定了经球孢白僵菌感染后红火蚁工蚁、蛹和幼蚁体内蛋白质含量的变化。结果表明: 红火蚁各虫态感染球孢白僵菌后体内蛋白质含量变化存在差异。在接种后12-72 h, 工蚁体内蛋白质含量在24 h时最高, 为47.12 mg/g, 显著低于对照的56.40 mg/g(P＜0.05), 此后呈下降趋势, 72 h时蛋白质含量下降至25.16 mg/g。幼蚁在接种36 h时体内蛋白质含量最高, 为24.13 mg/g, 此后呈下降趋势, 72 h时蛋白质含量为8.95 mg/g, 显著低于对照的24.80 mg/g。蛹感染球孢白僵菌后体内蛋白质含量一直呈下降趋势, 从12 h的36.57 mg/g降到72 h的10.42 mg/g, 与对照的38.61 mg/g相比差异显著(P＜0.05)。结果显示球孢白僵菌感染能显著降低红火蚁各虫态体内蛋白质含量。     

家蚕感染蛹虫草后的生理生化变化

蛹虫草分生孢子侵染5龄家蚕Bombyx mori后,家蚕血淋巴中总糖、海藻糖、蛋白质和甘油酯含量均有不同程度的下降,其中甘油酯含量下降最为明显。海藻糖酶活性在侵染初期也明显降低。接种后家蚕体内的保护酶超氧化物歧化酶、过氧化物酶和过氧化氢酶活性也有较大变化,其中超氧化物歧化酶活性上升最为明显,在4日内由441.841 U/mL升至601.255 U/mL。     

桃小食心虫危害对苹果果实蛋白质含量及防御酶活性的影响

为探明桃小食心虫取食危害对不同品种苹果果实蛋白质含量和防御酶活性的影响,田间条件下采用人工接虫和针刺模拟危害苹果果实,处理12 d后调查果实受害程度并测定蛋白质含量及超氧化物歧化酶(SOD)、过氧化物酶(POD)和过氧化氢酶(CAT)活性,分析了果实蛀孔数与可溶性蛋白质和防御性酶活性的关系。结果表明:人工接虫后,"嘎啦"的蛀孔数显著多于"乔纳金"和"金帅"。桃小食心虫危害后苹果果实蛋白质含量变化不大,均显著低于针刺模拟处理;SOD活性显著高于针刺模拟处理(P0.05);POD活性都显著增加,"乔纳金"、"金帅"的变化显著大于"嘎啦";CAT活性都与对照相比无显著变化,均高于针刺模拟处理,CAT酶活性与苹果蛀孔数呈显著正相关。桃小食心虫危害可以诱导寄主产生一系列反应,蛋白质含量和应激防御酶活性均发生了变化,其中,防御性酶可能在苹果防御桃小食心虫危害中发挥着重要作用。     

吸湿—回干处理降低番茄种子电解质渗漏的机理研究

对吸湿－回干处理降低番茄种子电解质渗漏的机理进行了研究,结果表明,吸湿－回干处理降低番茄种子电解质渗漏的效应产生于吸湿阶段。随吸湿时间延长,电解质渗漏下降,而ＳＯＤ、ＣＡＴ活性上升。mRNA和蛋白质合成抑制对剂电解质渗漏下降与ＳＯＤ、ＣＡＴ活性上升均无抑制作用,表明吸湿处理降低电解质渗漏、提高ＳＯＤ、ＣＡＴ活性的作用mＲＮＡ和蛋白质合成无关,吸湿和吸湿－回干处理后Ｋ３Ｆe(CN)6还原活显著下降,表明的生理生化状态发生了某种变化。     

前裂长管茧蜂寄生行为对桔小实蝇幼虫生理指标的影响

通过观察测定了桔小实蝇幼虫生长发育过程中血淋巴蛋白种类和血细胞的变化以及前裂长管茧蜂的寄生行为对桔小实蝇幼虫各项生理指标的影响。结果表明:不同日龄桔小实蝇幼虫的血细胞浓度随着虫龄的增加呈显著上升趋势,由2龄的16.53×106cells/mL,到3龄的30.14×106cells/mL直至蛹前期的35.94×106cells/mL,但血淋巴蛋白种类没有明显变化。和未寄生幼虫相比,寄生后的幼虫各类型血细胞的浓度均下降,但差异均不显著;血淋巴蛋白种类无明显增减,但浓度有所变化;寄生4 h后血淋巴蛋白质浓度显著降低,接近22 h时升高,至化蛹前期浓度再次下降;寄生行为使幼虫的发育历期从8 d延长至9～11d;4日龄幼虫在被寄生后的第4 d起体重显著高于未被寄生的桔小实蝇幼虫。     

茚虫威亚致死浓度对茚虫威敏感性降低的棉铃虫生物学参数及解毒酶活性的影响

【目的】本研究旨在明确茚虫威亚致死浓度对茚虫威敏感性降低的棉铃虫Helicoverpa armigera生物学参数及解毒酶活性的影响,以科学有效防治这一害虫,避免其对茚虫威的抗性快速发展。【方法】采用浸叶法测定了茚虫威对棉铃虫茚虫威抗性汰选种群(TP)及其同源对照种群(CP)3龄幼虫的毒力;用两性生命表分析LC₂₀浓度茚虫威对TP种群当代(F₀)生命表参数的影响,并测定了LC₂₀浓度茚虫威处理48 h后CP和TP种群棉铃虫3龄幼虫体内解毒酶［多功能氧化酶(MFO)、羧酸酯酶(CarE)和谷胱甘肽-S-转移酶(GST)］及乙酰胆碱酯酶(AChE)的活性。【结果】茚虫威对棉铃虫CP种群和TP种群3龄幼虫的LC₂₀分别为2.27和9.91 mg/L。LC₂₀茚虫威处理TP种群后,48 h的生长量、化蛹率、羽化率和成虫畸形率均显著低于未用药对照,而特定年龄生命期望值e_xj高于未用药对照;TP种群棉铃虫3龄幼虫体内GST和MFO活性与CP种群相比显著升高,CarE活性显著降低。【结论】本研究结果表明棉铃虫TP种群在LC₂₀浓度茚虫威胁迫下存在明显的生长与繁殖不利性,同时对其也产生了适应能力。LC₂₀浓度茚虫威处理后,棉铃虫TP种群的GST和MFO活性被显著诱导,说明这两种酶可能与棉铃虫对茚虫威产生抗药性密切相关;而CarE活性被显著抑制,说明该酶可能参与了茚虫威转化成N-脱甲氧羰基代谢物(DCJW)的活化过程。     

丽斗蟋翅二型雌虫飞行肌和卵巢发育间的资源分配差异

丽斗蟋Velarifictorus ornatus具有明显的翅二型现象, 长翅型与短翅型雌虫的卵巢和飞行肌存在着生理权衡。本研究分别应用蒽酮比色法、 硫代磷酸香草醛法、 考马斯亮蓝染液对羽化后10 d内两型雌虫飞行肌与卵巢内糖原、 总脂及蛋白质含量进行了定量分析。结果表明： 成虫羽化后10 d内, 两型雌虫体重无明显差异(P>0.05), 但短翅型雌虫怀卵量明显多于长翅型雌虫, 而人工脱翅能够促进长翅型雌虫怀卵量增加(P<0.05)。短翅型雌虫飞行肌内蛋白质、 糖原及总脂含量在成虫羽化后10 d内无明显变化, 但长翅型雌虫飞行肌内蛋白质在成虫羽化后3 d时达到最大值564.4±87.5 μg/♀, 糖原与总脂含量分别于羽化后第5天达到最大值85.2±21.7 μg/♀和5 284.7±1 267.4 μg/♀。然后开始下降, 各实验处理天数内, 长翅型雌虫飞行肌内蛋白质、 糖原及总脂含量都显著多于短翅型雌虫(P<0.05)。相反, 各处理天数内, 短翅型雌虫卵巢内蛋白质、 糖原及总脂含量则明显多于长翅型雌虫(P<0.05), 同时虫龄对蛋白质、 糖原及总脂在两型雌虫飞行肌与卵巢内分配也产生明显影响(P<0.05)。人工脱翅能够促进长翅型雌虫卵巢内蛋白质、 糖原及总脂含量增加, 同时诱导飞行肌内蛋白质、 糖原及总脂含量降低, 其中总脂含量在脱翅后10 d时降为2 394.9±1 461.8 μg/♀, 只有最大值的一半, 而与短翅型雌虫相似(P>0.05), 表明总脂为丽斗蟋飞行的主要能源物质。外用保幼激素Ⅲ能够促进长翅型雌虫卵巢内蛋白质、 糖原及总脂含量增加(P<0.05), 但对飞行肌内三者含量无明显影响(P>0.05), 外用早熟素Ⅰ对短翅型雌虫卵巢内蛋白质、 糖原及总脂含量亦无明显影响(P>0.05)。上述结果表明, 丽斗蟋长翅型雌虫首先将获得的资源用于发育飞行所需的飞行肌, 短翅型雌虫则首先将所获得的资源用于发育繁殖所需的卵巢, 但长翅型雌虫飞行肌与卵巢间的资源分配方式受保幼激素的影响。     

微囊藻毒素LR对人HL7702细胞蛋白磷酸酶2A的影响

微囊藻毒素能显著抑制蛋白磷酸酶2A的活性,是公认的一类肝毒素。为进一步研究微囊藻毒素作用于离体细胞后细胞中PP2A相关指标的变化,实验用不同浓度的MC-LR对人正常肝细胞HL7702染毒24h后检测细胞中PP2A亚基蛋白和mRNA水平,并检测3、6、12和24h作用后细胞内PP2A的酶活性。结果发现,除B55α蛋白表达有明显的下降趋势且1000 nmol/L组有显著性降低外,其他亚基的蛋白没有明显改变;15种PP2A亚基mRNA水平在100 nmol/L组都显著升高,而500和1000 nmol/L组分别有7种和6种亚基的mRNA表现出显著性降低。用不同浓度MC-LR染毒6h后,细胞内PP2A酶活有显著性降低,并且呈现剂量依赖性关系,而3、12和24h染毒后酶活性没有明显变化。以上结果表明:一定浓度的MC-LR作用24h后影响了HL7702细胞PP2A相关亚基的转录,但没有明显改变蛋白质水平;MC-LR对细胞内PP2A的酶活抑制作用与染毒时间密切相关。       

The effect of L-canavanine and L-canaline on the hemolymph amino acid composition of the tobacco hornworm,Manduca sexta (L.) (Sphingidae)

Tobacco hornworm larvae, Manduca sexta (L.) (Sphingidae), were administered L-canaline either by parenteral injection or by dietary consumption. The overt toxicity and the alteration of hemolymph amino acids caused by these nonprotein amino acids were evaluated. The LD₅₀ value for parenterally administered canavanine and canaline is 1.0 and 2.5 mg/g fresh body weight, respectively. A dietary concentration of 5.2 mM for canavanine and over 20 mM for canaline represent the respective LC₅₀ values. A large percentage of the larvae reared on diets supplemented with additional arginine, ornithine, or 2,4-diaminobutyric acid in addition to canavanine or canaline were unable to complete larval-pupal ecdysis. These toxic effects were associated with a decreased glutamic acid hemolymph titer and dramatically elevated ornithine. On the other hand, larvae administered canavanine or canaline alone, either by dietary consumption or parenteral injection, experienced less drastic developmental aberrations. These symptoms were in some cases correlated with increased ornithine and glutamic acid titers. Evidence is presented that even a canavanine- and canaline-sensitive insect such as M. sexta has a marked ability to eliminate these protective allelochemicals.     

A radiometric assay for determining the incorporation of L-canavanine or L-arginine into protein

Procedures for a radiometric assay of L-[guanidinooxy-14C]canavanine were developed which provide a convenient and accurate measure of the incorporation of [14C]canavanine into de novo-synthesized proteins. These methods are also applicable to determining [14C]arginine incorporation into protein. These procedures have been employed to study the synthesis of L-[guanidinooxy-14C]canavanine- and L-[guanidino-14C]arginine-containing proteins from the hemolymph of Manduca sexta and Heliothis virescens, two highly destructive insect pests.     

感染布氏白僵菌后油松毛虫血淋巴中海藻糖酶活性、海藻糖和葡萄糖含量的变化

为了揭示病原真菌白僵菌Beauveria侵染昆虫过程中如何利用虫体内糖类物质作为自身营养, 本研究测定了布氏白僵菌Beauveria brongniartii (Sacc.) Petch （2382菌株）感染油松毛虫Dendrolimus tabulaeformis Tsai et Liu幼虫后, 虫体血淋巴中酸性海藻糖降解酶活性及海藻糖和葡萄糖含量的变化。油松毛虫4龄幼虫感染菌株孢子悬浮液后, 血淋巴中酸性海藻糖降解酶的活性明显高于对照组, 感染后第3天酶活性达到最大值（0.2786 U/mg）, 此后第4-6 天酶活性逐渐降低; 染菌后的6 d中, 血淋巴中海藻糖含量显著低于对照组, 同样在感染后第4天其含量逐渐降低, 第6天时降到最低值。相比之下, 处理组血淋巴中的葡萄糖含量显著高于对照组; 处理组其含量在第1-3天内呈现快速升高趋势, 在第3天达到最大值（7.7615 mmol/L）, 然后逐渐降低。结果说明, 白僵菌侵入昆虫血淋巴后, 菌株代谢产生酸性海藻糖降解酶, 将血淋巴中的海藻糖水解成为葡萄糖, 然后为真菌利用, 破坏了虫体内的血糖平衡, 这是一个相互连接的生理代谢和生化反应过程。     

The effects of boric acid-induced oxidative stress on antioxidant enzymes and survivorship in Galleria mellonella

Larvae of the wax moth, Galleria mellonella (L.), were reared from first instar on a diet supplemented with 156, 620, 1,250, or 2,500 ppm boric acid (BA). The content of malondialdehyde (MDA, an oxidative stress indicator), and activities of the antioxidant enzymes [superoxide dismutase (SOD), catalase (CAT), glutathione S-transferase (GST), and glutathione peroxidase (GPx)] were determined in the fat body and hemolymph in the 7th instar larvae and newly emerged pupae. Relative to control larvae, MDA was significantly increased in larval hemolymph, larval and pupal fat body, but decreased in the pupal hemolymph. Insects reared on diets with 156- and 620-ppm BA doses yielded increased SOD activity but 1,250- and 2,500-ppm doses resulted in decreased SOD activity in larval hemolymph. SOD activity was significantly increased but CAT was decreased in the larval fat body. High dietary BA treatments led to significantly decreased GST activity. However, they increased GPx activity in larval hemolymph. Dietary BA also affected larval survival. The 1,250- and 2,500-ppm concentrations led to significantly increased larval and pupal mortality and prolonged development. In contrast, the lowest BA concentration increased longevity and shortened development. We infer that BA toxicity is related, at least in part, to oxidative stress management.     

Changes of acid phosphatase content and activity in the fat body and the hemolymph of the flesh fly Neobellieria (sarcophaga) bullata during metamorphosis

Changes in the specific and total activity of the lysosomal marker enzyme acid phosphatase (Acph) and in the amount of enzyme protein were examined in the fat body and the hemolymph from the last larval molt to the larval-pupal apolysis. The specific activity showed minor changes during the last larval period. In contrast, the total activity of the enzyme was low during the feeding period and higher during the wandering stage and strikingly increased at the time of puparium formation. We purified a protein having para-nitrophenyl phosphate phosphatase (Acph) activity and raised antisera against it. The amount of Acph protein in the fat body and hemolymph was examined using an ELISA. The specific Acph content showed little variation, but the total amount of the enzyme protein showed a stepwise increase in both organs during last larval stage and was markedly elevated in the pupal stage in the fat body. In contrast, a considerable decrease in the amount of Acph protein was observed in the hemolymph during this period. These data were in agreement with immunohistochemical observations showing an accumulation of the enzyme protein in fat body cells during the prepupal stage with a concomitant disappearance of the enzyme from the hemolymph. Inhibition of ecdysteroid secretion by water stress prevented the changes both in total enzyme activity and in the amount of Acph protein. However, Acph protein content and enzyme activity could be restored when the water stress was followed by a 20-hydroxyecdysone (20-HE) treatment. Taken together, our data show that Acph is secreted by fat body cells into the hemolymph during the larval stage, where it is stored in an inactive form. Increase in the 20-HE titer at the end of last larval stage reverses this process, and the enzyme is taken up by the fat body cells, where it becomes activated and appears in auto- and heterophagic vacuoles. Arch. Insect Biochem. Physiol. 34:369–390, 1997. © 1997 Wiley-Liss, Inc.     

Studies of L-canavanine incorporation into insectan lysozyme.

L-Canavanine is incorporated into the lysozyme synthesized, in response to administration of bacterial cell wall materials, by canavanine-treated larvae of the tobacco hornworm Manduca sexta (Sphingidae). Maximum canavanine incorporation into M. sexta lysozyme occurs when the larvae are provided 1 mg of canavanine g-1 fresh body weight. Analysis of canavanine-containing lysozyme purified from these insects reveals that 21% of the arginine residues are replaced by canavanine; this residue substitution results in a loss of 49.5% of the catalytic activity. When the larvae are provided 0.5 mg of canavanine g-1, 16.5% of the arginine residues are substituted by canavanine and 39.5% of the catalytic activity is lost. Canavanine is also incorporated into the lysozyme induced by canavanine-treated pupae of the giant silk moth Hyalophora cecropia (Saturnidae). In contrast, replacement of 17% of the arginine in H. cecropia lysozyme by canavanine fails to affect the catalytic activity. We have determined the primary structure of M. sexta lysozyme and compared it with the primary structure of H. cecropia lysozyme which has been described elsewhere. M. sexta lysozyme has an arginine at positions 23, 42, and 107. H. cecropia contains serine, lysine, and lysine, respectively, at these locations. The ability of incorporated canavanine to inhibit M. sexta lysozyme activity selectively may result from the fact that replacement of any one of the 3 arginine residues at position 23, 42, or 107 by canavanine causes the loss of catalytic activity.     

Biosynthesis of apolipophorin-III by the fat body in locusts

Biosynthesis of locust apolipophorin-III (apo-III) was studied in vitro. Gel electrophoresis and immunoblotting analyses of the locust hemolymph demonstrated that apo-III first appears in the hemolymph on the day 3 of the adult stage after the final molt and its hemolymph concentration increases thereafter. When incubated in vitro in a medium containing radioactive amino acid, the fat body cells synthesized the radiolabeled apo-III and released it into the medium. The developmental change in the apo-III synthesizing activity in the fat body reflected that of the apo-III concentration in the hemolymph. RNA isolated from the adult fat body directed the synthesis of apo-III as a major translation product in a cell-free system. These results indicate that the fat body is the tissue responsible for the synthesis of the locust apo-III, and biosynthesis of apo-III is developmentally regulated at the level of mRNA in accordance with the flight activity of the locust.     

急性低氧/复氧胁迫对克氏原螯虾抗氧化-能量代谢的影响

为研究低氧/复氧胁迫对克氏原螯虾(Procambarus clarkii)抗氧化及能量代谢的影响,将克氏原螯虾暴露于(1.0±0.1) mg/L急性低氧胁迫和后续(6.8±0.2) mg/L复氧环境中,于低氧胁迫1h、6h及复氧1h、12h分别采集肝胰腺、鳃和血淋巴,研究低氧/复氧胁迫下克氏原螯虾抗氧化-能量代谢酶的活力变化,分析鳃和肝胰腺组织的超微结构改变。在低氧胁迫下,肝胰腺和血淋巴中SOD酶活力显著下降(P<0.05);复氧以后,肝胰腺、血淋巴及鳃组织中SOD酶活力均出现了显著上升(P<0.05)。SOD酶活力变化可能与复氧过程中超氧阴离子自由基的过量产生有关。在复氧12h后,血淋巴和鳃组织中MDA含量均出现了显著性增加(P<0.01),提示机体细胞在复氧胁迫下产生了脂质过氧化。在低氧胁迫下,肝胰腺、鳃和血淋巴中ACP、AKP酶活力显著上升(P<0.05);在复氧12h后,肝胰腺和鳃组织中ACP酶活力显著降低(P<0.01)。显示低氧/复氧胁迫影响了机体的非特异性免疫应答。在急性低氧胁迫下,肝胰腺、血淋巴与鳃组织中的LDH含量和总ATPase活力均显...     

Lipid metabolism in the cockroach, Periplaneta americana, is activated by the hypertrehalosemic peptide, HTH-I

Phosphatidylcholine and phosphatidylethanolamine are the major constituents of the phospholipid pool in cockroach (Periplaneta americana) fat body and hemolymph. Both species of phospholipid are significantly decreased 6h after injecting hypertrehalosemic hormone I (HTH-I) into the hemocoel. Loss of phospholipid is accompanied by an accumulation of the phospholipid degradation products glycerophosphorylcholine and glycerol. HTH-I also increases phospholipase activity in the hemolymph and this is thought to be responsible for the depletion of hemolymph phospholipid. Phospholipase activity peaks approximately 2h after injection of HTH-I and returns to normal at 6h. In vitro, total phospholipid in the fat body is decreased by HTH-I whereas the concentration of diacylglycerol displays a corresponding increase. HTH-I elevates free fatty acid levels but has no effect on triacylglycerol. These effects of HTH-I are blocked by the phospholipase inhibitor mepacrine.     

Carbohydrate metabolism during starvation in the silkworm Bombyx mori

The effect of starvation on carbohydrate metabolism in the last instar larvae of the silkworm Bombyx mori was examined. Trehalose concentration in the hemolymph increased slightly during the first 6 h of starvation and decreased thereafter, whereas glucose concentration decreased rapidly immediately after diet deprivation. Starvation-induced hypertrehalosemia was completely inhibited by neck ligation, suggesting that starvation stimulates the release of a hypertrehalosemic factor(s) from the head. The percentage of active glycogen phosphorylase in the fat body increased within 3 h of starvation and its glycogen content decreased gradually. These observations suggest that production of trehalose from glycogen is enhanced in starved larvae. However, hypertrehalosemia during starvation cannot be explained by the increased supply of trehalose into hemolymph alone, as similar changes in phosphorylase activity and glycogen content in the fat body were observed in neck-ligated larvae, in which hemolymph trehalose concentration did not increase but decreased gradually. When injected into larvae, trehalose disappeared from hemolymph at a rate about 40% lower in starved larvae than neck-ligated larvae. The hemolymph lipid concentration increased during starvation, suggesting that an increased supply of lipids to tissues suppresses the consumption of hemolymph trehalose and this is an important factor in hypertrehalosemia.