光照对光生物反应器中微藻高密度光自养培养的影响

光生物反应器是实现微藻高密度培养的重要装置,其设计的关键技术之一是选择合适的光照方式。根据国内外近十年来的相关研究成果,重点介绍了入射光性质(光源、光强、光质和光暗循环)和光能分布对微藻生长的影响,评述了用于微藻高密度培养的光照技术,展望了进一步的研究方向,为高效光生物反应器的设计和优化提供参考。     

Cell Density and Cell Division in the Early Morphogenesis of the Chick Wing

THE early development of the chick wing involves cell differentiation, pattern formation and growth¹. In general terms, its morphogenesis can be seen in terms of how the growth of the mesenchyme and ectoderm is controlled, so that the very simple initial protrusion is transformed into an elongated paddle-like structure. At the same time a spatial pattern of differentiation must be specified within the mesenchyme, the cells forming cartilage and muscle so that the major skeletal and muscular features are laid down. In a previous paper² we described the changing pattern of the distribution of mitoses in the mesenchyme. We found that there was an overall fall in mitotic index from early stages (18–19 Hamburger-Hamilton) but that this occurred more rapidly in the proximal regions after about stage 23 so that a graded proximo-distal increase in mitotic index became established. We also suggested that the overall form was determined by the ectoderm and not the mesenchyme. This raised specific problems about the control of growth of the mesenchyme: we could not account for the observed distribution of mitoses but wondered whether this involved a temporal programme or was related to positional information. Our investigations of the so-called mesenchymal condensations which are supposed to be the prelude to cartilage formation³ have led to detailed analysis of cell density during early morphogenesis. We show here that the cell density varies in a very regular manner and is closely correlated with mitotic index: mitotic index is inversely proportional to cell density. This finding is not only important in its own right because it may be the first demonstration of density dependent growth control⁴in vivo, but because it provides a new mechanism for the control of growth and pattern formation in limb morphogenesis.     

Density Gradient Centrifugation Compromises Bone Marrow Mononuclear Cell Yield

Bone marrow mononuclear cells (BMNCs) are widely used in regenerative medicine, but recent data suggests that the isolation of BMNCs by commonly used Ficoll-Paque density gradient centrifugation (DGC) causes significant cell loss and influences graft function. The objective of this study was to determine in an animal study whether and how Ficoll-Paque DGC affects the yield and composition of BMNCs compared to alternative isolation methods such as adjusted Percoll DGC or immunomagnetic separation of polymorphonuclear cells (PMNs). Each isolation procedure was confounded by a significant loss of BMNCs that was maximal after Ficoll-Paque DGC, moderate after adjusted Percoll DGC and least after immunomagnetic PMN depletion (25.6±5.8%, 51.5±2.3 and 72.3±6.7% recovery of total BMNCs in lysed bone marrow). Interestingly, proportions of BMNC subpopulations resembled those of lysed bone marrow indicating symmetric BMNC loss independent from the isolation protocol. Hematopoietic stem cell (HSC) content, determined by colony-forming units for granulocytes-macrophages (CFU-GM), was significantly reduced after Ficoll-Paque DGC compared to Percoll DGC and immunomagnetic PMN depletion. Finally, in a proof-of-concept study, we successfully applied the protocol for BMNC isolation by immunodepletion to fresh human bone marrow aspirates. Our findings indicate that the common method to isolate BMNCs in both preclinical and clinical research can be considerably improved by replacing Ficoll-Paque DGC with adapted Percoll DGC, or particularly by immunodepletion of PMNs.     

Effects of Malaria Parasite Density on Blood Cell Parameters

Changes in blood cell parameters are already a well-known feature of malarial infections. To add to this information, the objective of this study was to investigate the varying effects that different levels of parasite density have on blood cell parameters. Patients diagnosed with malaria at Phobphra Hospital, Tak Province, Thailand between January 1^st 2009 and January 1^st 2012 were recruited as subjects for data collection. Blood cell parameters of 2,024 malaria-infected patients were evaluated and statistically analyzed. Neutrophil and platelet counts were significantly higher, however, RBC count was significantly lower in patients with P. falciparum infection compared to those with P. vivax infection (p<0.0001). Leukocyte counts were also significantly higher in patients with high parasitemia compared to those with low and moderate parasitemia. In terms of differential leukocyte count, neutrophil count was significantly higher in patients with high parasitemia compared to those with low and moderate parasitemia (p<0.0001). On the other hand, both lymphocyte and monocyte counts were significantly lower in patients with high parasitemia (p<0.0001). RBC count and Hb concentration, as well as platelet count were also significantly reduced (p<0.05) and (p<0.0001), respectively. To summarize, patients infected with different malaria parasites exhibited important distinctive hematological parameters, with neutrophil and eosinophil counts being the two hematological parameters most affected. In addition, patients infected with different malarial densities also exhibited important changes in leukocyte count, platelet count and hemoglobin concentration during the infection. These findings offer the opportunity to recognize and diagnose malaria related anemia, help support the treatment thereof, as well as relieve symptoms of severe malaria in endemic regions.     

134 Cryopreservation of Chlamydomonas Reinhardtii (Chlorophyceae): A Cause of Low Viability at High Cell Density

Cryopreservation provides a convenient method for long term storage of living organisms. Current protocols allow the successful cryopreservation of a wide range of algae, although many strains remain recalcitrant to cryopreservation. Chlamydomonas reinhardtii , a species utilized in many molecular and biochemical studies, survives cryopreservation best at low cell density. We show that reduced viability at higher cell densities is caused by the accumulation of a substance released from C. reinhardtii into the culture medium during cryopreservation. A mutant strain of C. reinhardtii (cw10) with a greatly reduced cell wall did not release a substance inhibitory to wild type or cw10 C. reinhardtii during cryopreservation, and could be cryopreserved with the same viability regardless of cell density. The inhibitory substance is small (mw<1300), polar, heat-stable and organic. Chlamydomonas moewusii Gerloff and Chlamydomonas zebra Korschikov ex Pascher both produce substances that reduce the viability of cryopreserved C. reinhardtii . However, neither is affected by the inhibitory substance produced by themselves or C. rienhardtii. Pandorina morum (Müller) Bory and Volvox carteri f. nagariensis Iyengar are colonial Volvocalean algae related to C. reinhardtii that cannot be successfully cryopreserved. They both generate substances that inhibit C. reinhardtii during cryopreservation. The identification of the substance inhibitory to C. reinhardtii during cryopreservation should explain why this alga cryopreserves best at a low cell density, and may lead to protocols that facilitate the more successful cryopreservation of C. reinhardtii and related algae.     

重组酵母菌的高密度发酵表达

酵母作为一类外源基因的表达系统具有很多优点 ,有许多外源基因在工程酵母菌表达生产重要的外源蛋白[1] 。从生理学角度看 ,作为外源基因的受体细胞 ,酵母的生理和遗传特性影响着外源基因的表达。同时 ,外源基因的表达 ,特别是高表达的外源蛋白对宿主细胞有抑制作用甚至会导致细胞中毒或死亡。再加上工程菌的培养过程中的不稳定性问题的存在 ,因此 ,菌体细胞的高浓度和目的基因的高表达是一对矛盾 ,它们互相制约 ,构成生物工程研究的重要工作之一。1 .工程酵母菌的高密度发酵酵母的高密度发酵是一个相对概念 ,一般指发酵液中酵母浓度在 30 …     

植物乳杆菌Lp-2的高密度发酵

高密度培养植物乳杆菌是制作其发酵剂的重要环节。首先,研究了不同的溶氧和pH对植物乳杆菌的分批发酵的影响。在分批发酵的基础上,为进一步提高发酵液中的菌体浓度,进行了补料分批发酵实验。最终通过对蔗糖反馈补料发酵试验对比改造获得了pH反馈补料发酵工艺。此发酵补料工艺可以控制蔗糖残糖量始终处于较低的水平,因此获得了最高的菌体产量。菌体干重达到13.56g/L,较分批培养提高90.05%。     

Effect of Cell Density on Thermotaxis of Paramecium1

ABSTRACT. The swiftness of thermotaxis of Paramecium caudatum has been investigated for various populations of organisms by measuring the transient spatial distribution of the gathering process of organisms that are transferred to a temperature-gradient cell from the culture medium. The dispersion obtained from the spatial distribution for each population is found to decrease linearly with time and finally reach a steady state value. The gathering rate determined by the slope of the dispersion strongly depends on population; it increases with population.     

Modulation of the Plasminogen Activator Activity of a Transformed Cell Line by Cell Density

The effects of variations in cell density on the expression of the plasminogen activator activity of a tumorigenic rat cell line were analyzed. At low cell densities, the plasminogen activator activity per cell was high and independent of cell density. As the cell density increased, the plasminogen activator activity per cell decreased until it eventually became inversely proportional to cell density. Inhibition of the plasminogen activator activity per cell by increases in cell density was not the result of the presence of a soluble inhibitor but seemed to require cell-to-cell contact. The V_max per cell for the activation of plasminogen changed at high cell densities, but the K_m did not change. This change in the V_max per cell was in part the result of a change in the catalytic rate constant for the conversion of plasminogen to plasmin. This was inferred from studies on the kinetics of inhibition of plasminogen activator activity by diisopropyl fluorophosphate as a function of cell density. For cells growing at high densities, the rate of inhibition was constant, exhibiting a second-order rate constant of 2.6 × 10⁻²M⁻¹ s⁻¹. For cells growing at low densities, the plasminogen activator activity was inhibited at two different rates, one exhibiting a second-order rate constant of 2.6 × 10⁻²M⁻¹ s⁻¹ and the other exhibiting a second-order rate constant of 9.4 × 10⁻²M⁻¹ s⁻¹. We discuss the importance of cell density in assays of the plasminogen activator activity of cells, the use of this cell line to study the biochemical basis of the density dependence of plasminogen activator activity, and the density-dependent role of plasminogen activator activity in tumor formation and metastasis.     

Substrate Compliance versus Ligand Density in Cell on Gel Responses

Substrate stiffness is emerging as an important physical factor in the response of many cell types. In agreement with findings on other anchorage-dependent cell lineages, aortic smooth muscle cells are found to spread and organize their cytoskeleton and focal adhesions much more so on “rigid” glass or “stiff” gels than on “soft” gels. Whereas these cells generally show maximal spreading on intermediate collagen densities, the limited spreading on soft gels is surprisingly insensitive to adhesive ligand density. Bell-shaped cell spreading curves encompassing all substrates are modeled by simple functions that couple ligand density to substrate stiffness. Although smooth muscle cells spread minimally on soft gels regardless of collagen, GFP-actin gives a slight overexpression of total actin that can override the soft gel response and drive spreading; GFP and GFP-paxillin do not have the same effect. The GFP-actin cells invariably show an organized filamentous cytoskeleton and clearly indicate that the cytoskeleton is at least one structural node in a signaling network that can override spreading limits typically dictated by soft gels. Based on such results, we hypothesize a central structural role for the cytoskeleton in driving the membrane outward during spreading whereas adhesion reinforces the spreading.     

Probability Density Function of the Red Cell Membrane Permeability Coefficient

The distribution of a random variable is determined by the probability density functions (PDF) of all other random variables with which the variable in question is jointly distributed. If the PDF of the random variable of interest is normal, or skewed normal, then the distributions with which it is jointly distributed determine its mean and standard deviation. In the case described here (where hemolysis time of the red blood cell is a function of the permeability coefficient and geometric variables of the cell) the mean and standard deviation of the permeability coefficient and the known distributions of the geometric variables on which the hemolysis time depends determine a predicted distribution of hemolysis time. An observed distribution of the hemolysis time is obtained spectrophotometrically. By choosing the mean and standard deviation of the permeability coefficient so that the predicted PDF of the hemolysis time matches the observed PDF best by least-squares criterion, the complete distribution of the permeability coefficient is determined.     

双碳源单细胞蛋白高密度培养

单细胞蛋白(SCP)培养具有增殖速度快、原料来源广、蛋白质含量高等优点,正在成为重要的蛋白质来源之一。生产SCP的原料包括烷烃、低碳醇类及碳水化合物。由碳水化合物,尤其是由各种农副产品加工的废料、造纸工业废水及木质纤维素水解产物等,生产SCP属于废弃资源的综合利用,具有重要的经济和社会意义。这类原料中常含有多种碳源,例如,在木质纤维水解液中,有以木糖为主的五碳糖,也有以葡萄糖为主的六碳糖,木糖与葡萄糖之比约为1:2。这样,木糖的利用就成了一个关键问题。葡萄糖对木糖代谢的抑制作用随葡萄糖比例的降低而减轻;Slinger和Bothast研究了用混合糖培养Candida shehetane的过程,当木糖与葡萄糖的比例为3:1及1:1时,葡萄糖的利用速度分别比木糖高1.6倍及3.4倍;在低还原势时,酵母产酒精速率降低而细胞增长速率加快,可以达到较高细胞浓度。     

Electric Field-Induced Transmembrane Potential Depends on Cell Density and Organizatio

Electrochemotherapy is a novel technique to enhance the delivery of chemotherapeutic drugs into tumor cells. In this procedure, electric pulses are delivered to cancerous cells, which induce membrane permeabilization, to facilitate the passage of cytotoxic drugs through the cell membrane. This study examines how electric fields interact with and polarize a system of cells. Specifically, we consider how cell density and organization impact on induced cell transmembrane potential due to an external electric field. First, in an infinite volume of spherical cells, we examined how cell packing density impacts on induced transmembrane potential. With high cell density, we found that maximum induced transmembrane potential is suppressed and that the transmembrane potential distribution is altered. Second, we considered how orientation of cell sheets and strands, relative to the applied field, affects induced transmembrane potential. Cells that are parallel to the field direction suppress induced transmembrane potential, and those that lie perpendicular to the applied field potentiate its effect. Generally, we found that both cell density and cell organization are very important in determining the induced transmembrane potential resulting from an applied electric field.     

脯氨酰内肽酶培养条件的优化及高密度发酵

基因工程菌E.coliBL21/pGEMPEP可以组成型表达重组的点状产气单胞菌脯氨酰内肽酶(PEP),但培养条件极大地影响着酶的产量,为了获得高效表达,首先测定了工程菌表达PEP的稳定性并考察了培养温度、pH、发酵时间、碳源、氮源、无机盐等对产酶的影响,得到了优化的发酵条件,L9(3⁴)正交试验进一步明确了摇床转速、培养温度、pH值、培养时间对产酶量的影响都有高度的统计学意义。在此基础上利用NBSBioFlo3000型5L自控发酵罐进行了高密度、高表达发酵、经20h培养,最终菌体密度达OD₆₀₀60(相当于干菌体225g/L),PEP表达量为28%,每升发酵液中含PEP酶315g。     

Bacterial Predator-Prey Interaction at Low Prey Density

A bacterial predator-prey interaction was studied using Bdellovibrio and bioluminescent prey bacteria. The attacking bdellovibrio causes decay of bioluminescence, which is correlated with bdellovibrio penetration into the prey. The behavior of the prey and predator populations over time was found to be well described by a Lotka-Volterra model. By using this model, the probability of bdellovibrio penetration after encountering a prey cell was found to be approximately 3.0%. The prey density required to give the bdellovibrios a 50% chance of survival was calculated to be at least 3.0 × 10⁶ cells per ml, and the density required for population equilibria was calculated to be about 7 × 10⁵ prey bacteria per ml. These values, not generally characteristic of natural habitats, suggest that the existence of Bdellovibrio in nature is limited to special ecological niches.