试管棉纤维与天然棉纤维超微结构的差异（简报）

Native cotton fiber and in vitro cotton fiber that was induced from cotton ovule callus by suspension culture were observed using transmission electron microscope and scanning electron microscope. The ovule surface on the first day preanthesis was quite smooth. On the anthesis, it had a lot of protuberances. Two kinds of callus, smooth and rough were found. The microfibrils of callus was vertical to the cell long axis and they changed their orientations with the development of the in vitro cotton fiber: from the vertical to shallow spiral and then to parallel to the cell long axis. So was the native cotton fiber. It suggests that in vitro cotton fiber and native cotton fiber have similar development process. Compared with the ovule surface cell, most callus cells had smaller nuclear. During the development of the fiber, the plasm of native cotton fiber was denser than that of in vitro fiber, and it has more cellular organ than in vitro fiber. The cell wall of native cotton fiber was thicker and denser than that of the in vitro cotton fiber too. It suggests that the physiological activity of in vitro cotton fiber was less active than native cotton fiber.     

Plant density influences fiber sucrose metabolism in relation to cotton fiber quality

Planting density plays an important role in improving cotton yield and regulating fiber quality. A 2-year experiment was conducted to investigate the effects of plant density on sucrose metabolism in relation to fiber quality of field-grown cotton. The results showed that lint yield increased with increasing plant density, fiber micronaire, fiber maturity ratio, and fiber fineness decreased with the increasing of plant density, whereas fiber length, fiber uniformity index, fiber strength, and fiber elongation were little affected by plant density. Increased plant density decreased sucrose synthase (SuSy) activity, sucrose content, and cellulose content in cotton fiber, but increased invertase activity. Increased invertase activity would restrain SuSy activity in cotton fiber: therefore, SuSy activity was the most severely affected enzyme in fiber sucrose metabolism by cotton plant density during fiber development. Abundant sucrose content in fiber after 24 days post anthesis (DPA) and high activities of SuSy and sucrose phosphate synthase (SPS) at 38 DPA were beneficial for cellulose synthesis, and were propitious to optimize the fiber maturity properties. The results also showed that fiber micronaire, maturity ratio, and fineness decreased 0.11, 0.02, and 5.89 mtex, respectively, with each increase of 10,000 plants per hectare. It was concluded that high plant density decreased SuSy activity, sucrose content, and cellulose content, but increased invertase activity in sucrose metabolism, resulting in low fiber micronaire, fiber maturity ratio, and fiber fineness.     

Dietary fiber

Dietary fiber is plant-derived material that is resistant to digestion by human alimentary enzymes. Fiber may be divided into two broad chemical classes: 1) non-alpha-glucan polysaccharides (cellulose, hemicelluloses, and pectins) and 2) lignins. Dietary fiber behaves within the gastrointestinal tract as a polymer matrix with variable physicochemical properties including susceptibility to bacterial fermentation, water-holding capacity, cation-exchange, and adsorptive functions. These properties determine physiological actions of fiber and are dependent on the physical and chemical composition of the fiber. Fiber undergoes compositional changes as a consequence of bacterial enzymatic action in the colon. Dietary fiber is of clinical significance in certain disorders of colonic function and in glucose and lipid metabolism. Dietary fiber increases stool bulk by acting as a vehicle for fecal water and by increasing fecal bacterial volume. Use of fiber in the treatment of constipation and uncomplicated diverticular disease is well established. By increasing stool bulk, fiber also reduces the fecal concentration of bile acids and other substances. Certain types of fiber decrease the rate of glucose absorption and attenuate postprandial rises in blood glucose and insulin. Plasma cholesterol levels are reduced by mucilaginous forms of fiber. This effect appears to be mediated in part by an increase in fecal acidic sterol excretion.     

Genotypic differences in some physiological characteristics during cotton fiber thickening and its influence on fiber strength

Cotton (Gossypium L.) fiber strength is linked with many complex physiological and biochemical processes in the stage of secondary fiber cell wall thickening. With the aim of further exploiting of the relationship between fiber strength and genotypic differences in physiological characteristics, the experiment was implemented in Nanjing, China (in the lower reach of Yangtze River Valley in China) at the stage of cotton fiber thickening stage in 2004–2005. The result showed that the higher strength fiber (genotype Kemian 1) always had higher activities of sucrose synthetase (SuSy) and β-1,3-glucan synthase, and more sucrose and callose existed and transformed for cellulose synthesis than these of the other genotypes during the fiber secondary wall thickening period These resulted in a longer and more gently cellulose accumulation and wider range and longer period of fiber strength enhancing. Interestingly, the opposite effects were observed in lower strength fiber of Dexiamian 1 and intermediary indices were found in NuCOTN 33B with middle strength fiber. Taken together, above results suggested the variations in the transformation of sucrose and callose contents, and the dynamics of sucrose synthase and β-1,3-glucan synthase activities, might be one of the physiological reasons causing the differences in the speed of cellulose accumulation and fiber strength formation. Additionally, other results showed: (1) the occurrence of callose content peak might be an important sign of the onset of the secondary wall thickening in the fiber cell; (2) the duration and the maximum growth rate of cellulose rapid accumulation contribute more to fiber strength development than other indices of cellulose rapid accumulation.     

Effect of fiber diameter on the behavior of biofilm and anodic performance of fiber electrodes in microbial fuel cells

A series of fiber electrodes with fiber diameters ranging from about 10 to 0.1 μm were tested as anodes in microbial fuel cells to study the effect of fiber diameter on the behavior of biofilm and anodic performance of fiber electrodes. A simple method of biofilm fixation and dehydration was developed for biofilm morphology characterization. Results showed that the current density of fiber anodes increased until the fiber diameter approached 1 μm which was about the length of the dominant microorganisms in biofilm. The highest current density was 3.08 mA cm(-2), which was obtained from fiber anode with high porosity of over 99% and fiber diameter of 0.87 μm. It was believed that the high current density was attributed to the high porosity, as well as proper fiber diameter which ensured formation of thick and continuous solid biofilms.     

Optimum fiber spacing in a hollow fiber bioreactor

A high surface area hollow fiber reactor was developed for mammalian cell culture. The reactor employs an interfiber gel matrix of agar or collagen for cell support. A model was developed to predict cell density as a function of fiber spacing. Optimum spacings are calculated for two sizes of Celgard hollow fibers. Ehrlich Ascites Tumor (EAT) cells were grown to an estimated density of 1.1 x 10(8) viable cells/mL in the extracapillary space-corresponding to an overall reactor density of 7 x 10(7) cells/mL. On the basis of available kinetic and diffusivity data, the model predicts that lactate accumulation may limit cell growth in the early stage of medium utilization, while oxygen delivery becomes limiting at later stages.     

Quantitative evaluation of threshold fiber strain that induces reorganization of cytoskeletal actin fiber structure in osteoblastic cells

The cytoskeletal stress fiber structure plays essential roles in various kinds of cellular functions such as shape maintenance, active motility and mechanosensing, and its structure is dynamically reorganized under each functional process. In known reorganization mechanisms of the stress fibers, a change in its mechanical condition has been suggested as one of the key mediators that affect the reorganization process. Some experimental studies have clarified that tension release in the stress fibers induces fiber depolymerization that is considered to be the initial phase of the reorganization process. However, quantitative mechanical values such as strain or stress that induce depolymerization have still not been evaluated. This study is aimed at the quantitative evaluation of the mechanical value that induces stress fiber depolymerization, to gain a basic understanding of the reorganization phenomenon from a mechanical viewpoint. Osteoblastic cells (MC3T3-E1) were cultured on prestretched silicone rubber substrate. Compressive deformation was applied to the cells by uniaxially releasing the prestretched substrate strain and change in the stress fiber structure was observed. The results indicated that the compressive strain magnitude, not in the whole cell body but in the stress fiber itself, is important to induce disassembly of the stress fiber structure. The existence of a threshold strain magnitude for initiating fiber disassembly was also suggested; the threshold strain magnitude was evaluated as approximately -0.20.     

Microbial hollow fiber bioreactors

Hollow fiber membranes have been used for more than a decade to culture mammalian cells and immobilize enzymes. More recently, hollow fiber bioreactors have shown encouraging potential for culturing microbes but many of the practical aspects of their operation have not been explored.     

Transitions of muscle fiber phenotypic profiles

Skeletal muscle is a complex, versatile tissue composed of a large variety of functionally diverse fiber types. The overall properties of a muscle largely result from a combination of the individual properties of its different fiber types and their proportions. Skeletal muscle fiber types, which can be delineated according to various parameters, for example, myofibrillar protein isoforms, metabolic enzyme profiles, and structural and contractile properties, are not fixed units but are capable of responding to altered functional demands and a variety of signals by changing their phenotypic profiles. This brief review summarizes our current understanding of the delineation of fiber types, modulations of their phenotypic profiles as induced under various conditions, and potential mechanisms involved in these transitions.     

Relation between muscle fiber conduction velocity and fiber size in neuromuscular disorders.

To determine the relation between muscle fiber conduction velocity (MFCV) and muscle fiber diameter (MFD) in pathological conditions, we correlated invasively measured MFCV values with MFD data obtained from muscle needle biopsies in 96 patients with various neuromuscular disorders. MFCV was significantly correlated with MFD and independent of the underlying disorder. Pathological diameter changes were fiber-type dependent, with corresponding MFCVs. A linear equation expresses the relation well: MFCV (m/s)=0.043.MFD (microm)+0.83. We conclude that fiber diameter determines MFCV largely independent of the underlying neuromuscular disorders studied.     

New insights into elastic fiber assembly

Elastic fibers provide recoil to tissues that undergo repeated stretch, such as the large arteries and lung. These large extracellular matrix (ECM) structures contain numerous components, and our understanding of elastic fiber assembly is changing as we learn more about the various molecules associated with the assembly process. The main components of elastic fibers are elastin and microfibrils. Elastin makes up the bulk of the mature fiber and is encoded by a single gene. Microfibrils consist mainly of fibrillin, but also contain or associate with proteins such as microfibril associated glycoproteins (MAGPs), fibulins, and EMILIN-1. Microfibrils were thought to facilitate alignment of elastin monomers prior to cross-linking by lysyl oxidase (LOX). We now know that their role, as well as the overall assembly process, is more complex. Elastic fiber formation involves elaborate spatial and temporal regulation of all of the involved proteins and is difficult to recapitulate in adult tissues. This report summarizes the known interactions between elastin and the microfibrillar proteins and their role in elastic fiber assembly based on in vitro studies and evidence from knockout mice. We also propose a model of elastic fiber assembly based on the current data that incorporates interactions between elastin, LOXs, fibulins and the microfibril, as well as the pivotal role played by cells in structuring the final functional fiber.     

Nucleolar size at early stages of cotton fiber development in relation to final fiber dimension

Changes in nucleolar size and nucleolar vacuolation at early stages of fiber development and final fiber dimensions were determined for cotton of different species: Gossypium hirsutum L. cv. B49, Gossypium barbadense L. cv. Menoufi and Gossypium arboreum L. cv. Virnar. Size of the nucleolus in combination with its vacuolation at an early stage of development was found to be clearly associated with the final result of fiber development.     

Structured fiber supports for gas phase biocatalysis

Pseudomonas cepaciae lipase adsorbed onto non-porous structured fiber supports in the form of woven fabrics, was used to catalyze hydrolysis and transesterification reactions in the gas phase. The enzyme adsorbed onto carbon fiber support exhibited much higher catalytic activity compared to the enzyme immobilized onto glass fiber carrier. The effect of temperature and relative humidity on reactions catalyzed by P. cepaciae lipase adsorbed onto structured fiber carbon support was studied in the gas system. Under the conditions investigated (up to 60 °C and 80% relative humidity), the immobilized enzyme showed a high thermostability and could be efficiently used to catalyze hydrolytic and transesterification reactions in continuous mode. Structured fiber supports, with a high specific surface area and a high mechanical resistance, showed a low-pressure drop during the passage of reactants through a reactor. The approach proposed in this study could be suitable for immobilization of a wide variety of enzymes.     

Xyloglucan breakdown during cotton fiber development

Cotton (Gossypium herbaceum L.) fibers elongated almost linearly up to about 20 days post anthesis. The molecular mass of xyloglucans in fiber cell walls decreased gradually during the elongation stage. When enzymatically active (native) cell wall preparations of fibers were autolyzed, the molecular mass of xyloglucans decreased. The decrease was most prominent in wall preparations obtained from the rapidly elongating fibers. The xyloglucan-degrading activity was recovered from the fiber cell walls with 3 mol/L NaCl, and the activity was high at the stages in which fibers elongated vigorously. These results suggest the possible involvement of xyloglucan metabolism in the regulation of cotton fiber elongation.     

Physiological and metabolic effects of dietary fiber

William Beaumont noted the gastric effects of vegetable fiber and suggested that dietary fiber may provide health benefits. In the last decade investigators documented the physiological effects of fiber on gastric emptying, intestinal nutrient absorption rates, and colon function. Further clinical investigation and much more of the type of repetitive observations pioneered by Beaumont are required to definitively establish the physiological effects of fiber on gastrointestinal physiology. High-fiber intake provides well-established benefits for persons with diabetes: it lowers insulin requirements, provides better control of blood glucose, and reduces serum lipids. Foods rich in soluble fiber, such as oat or bean products, lower cholesterol significantly for persons with hypercholesterolemia and for healthy young subjects. High-fiber foods also lower serum triglycerides and blood pressure. Several studies indicate that high intake of fiber protects against coronary heart disease.     

Composition and structure study of natural Nelumbo nucifera fiber

Nelumbo nucifera (Nn.) fiber is the isolated secondary wall of the Nn. leafstalk Tracheary elements which has a unique shape. As the shape of the fiber may strongly affect the industrial uses especially for textile usage, the morphology and structure of Nn. fiber at different growth stages were investigated by several techniques in the present work. The Nn. fiber has spriral morphology with cellulose I structure. The diameter of mature fiber is about 4 μm and the cross-section shows elliptical or slightly oval shape without lumen. These findings aim to deeply understand the structure of Nn. fiber which is expected to be helpful to bring Nn. fiber into industrial use.     

Microfibril-associated MAGP-2 stimulates elastic fiber assembly

Elastic fibers are complex structures composed of a tropoelastin inner core and microfibril outer mantle guiding tropoelastin deposition. Microfibrillar proteins mainly include fibrillins and microfibril-associated glycoproteins (MAGPs). MAGP-2 exhibits developmental expression peaking at elastic fiber onset, suggesting that MAGP-2 mediates elastic fiber assembly. To determine whether MAGP-2 regulates elastic fiber assembly, we used an in vitro model featuring doxycycline-regulated cells conditionally overexpressing exogenous MAGP-2 and constitutively expressing enhanced green fluorescent protein-tagged tropoelastin. Analysis by immunofluorescent staining showed that MAGP-2 overexpression dramatically increased elastic fibers levels, independently of extracellular levels of soluble tropoelastin, indicating that MAGP-2 stimulates elastic fiber assembly. This was associated with increased levels of matrix-associated MAGP-2. Electron microscopy showed that MAGP-2 specifically associates with microfibrils and that elastin globules primarily colocalize with MAGP-2-associated microfibrils, suggesting that microfibril-associated MAGP-2 facilitates elastic fiber assembly. MAGP-2 overexpression did not change levels of matrix-associated fibrillin-1, MAGP-1, fibulin-2, fibulin-5, or emilin-1, suggesting that microfibrils and other elastic fiber-associated proteins known to regulate elastogenesis do not mediate MAGP-2-induced elastic fiber assembly. Moreover, mutation analysis showed that MAGP-2 does not stimulate elastic fiber assembly through its RGD motif, suggesting that integrin receptor binding does not mediate MAGP-2-induced elastic fiber assembly. Because MAGP-2 interacts with Jagged-1 that controls cell-matrix interaction and cell motility, two key factors in elastic fiber macroassembly, microfibril-associated MAGP-2 may stimulate elastic fiber macroassembly by targeting the release of elastin globules from the cell membrane onto developing elastic fibers.