定价： 481元 / 折扣价： 409 元 加购物车

定价： 605元 / 折扣价： 515 元 加购物车

定价： 571元 加购物车

定价： 571元 加购物车

定价： 646元 加购物车

定价： 590元 加购物车

4.1 The composition and sequential structure of alginate, as well as the molar mass and molar mass distribution, determines the functionality of alginate in an application. For instance, the gelling properties of an alginate are highly dependent upon the composition and molar mass of the polymer.4.2 Light scattering is one of very few methods available for the determination of absolute molar mass and structure, and it is applicable over the broadest range of molar masses of any method. Combining light scattering detection with size exclusion chromatography (SEC), which sorts molecules according to size, gives the ability to analyze polydisperse samples, as well as to obtain information on branching and molecular conformation. This means that both the number-average and mass-average values for molar mass and size may be obtained for most samples. Furthermore, one has the ability to calculate the distributions of the molar masses and sizes.4.3 Multi-angle laser light scattering (MALS) is a technique where measurements are made simultaneously over a range of different angles and used to determine the scattering at 0°, which directly relates to molecular weight. MALS detection can be used to obtain information on molecular size, since this parameter is determined by the angular variation of the scattered light. This can be related to branching, aggregation, and molecular conformation. Molar mass can also be determined by detecting scattered light at a single low angle (LALS) and assuming that this is not significantly different from the scattering at 0°.4.4 Size exclusion chromatography uses columns, which are typically packed with polymer particles containing a network of uniform pores into which solute and solvent molecules can diffuse. While in the pores, molecules are effectively trapped and removed from the flow of the mobile phase. The average residence time in the pores depends upon the size of the solute molecules. Molecules that are larger than the average pore size of the packing are excluded and experience virtually no retention; these are eluted first, in the void volume of the column. Molecules which penetrate the pores will have a larger volume available for diffusion; their retention will depend on their molecular size, with the smaller molecules eluting last.4.5 For polyelectrolytes, dialysis against the elution buffer has been suggested, in order to eliminate Donnan-type artifacts in the molar mass determination by light scattering (1, 2).6 However, in the present method, the size exclusion chromatography step preceding the light scatter detection is an efficient substitute for a dialysis step. The sample is separated on SEC columns with large excess of elution buffer for 30 to 40 min, and it is therefore in full equilibrium with the elution buffer when it reaches the MALS detector.1.1 This test method covers the determination of the molar mass (typically expressed as grams/mole) of sodium alginate intended for use in biomedical and pharmaceutical applications as well as in tissue-engineered medical products (TEMPs) by size exclusion chromatography with multi-angle laser light scattering detection (SEC-MALS). A guide for the characterization of alginate has been published as Guide F2064.1.2 Alginate used in TEMPs should be well characterized, including the molar mass and polydispersity (molar mass distribution) in order to ensure uniformity and correct functionality in the final product. This test method will assist end users in choosing the correct alginate for their particular application. Alginate may have utility as a scaffold or matrix material for TEMPs, in cell and tissue encapsulation applications, and in drug delivery formulations.1.3 The values stated in SI units are to be regarded as standard. No other units of measurement are included in this standard.1.4 This standard does not purport to address all of the safety concerns, if any, associated with its use. It is the responsibility of the user of this standard to establish appropriate safety and health practices and determine the applicability of regulatory limitations prior to use.

定价： 590元 加购物车

This specification establishes the requirements and test methods for the materials, dimensions, workmanship, and finished quality of injection molded polyvinyl chloride (PVC) profile sections used for the field fabrication of a PVC liner inside existing man-entry size circular and non-circular sewers; circular, non-circular, and box culverts, conduits, and vertical shafts or manholes having dimensions of 39.4 in. and larger (1000 mm and larger). It covers segmental panel system for non-pressure applications where the PVC liner is installed in the existing structure and the annular space between the liner and the existing structure is grouted with a low viscosity, high strength cementitious grout.1.1 This specification covers the requirements and test methods for the materials, dimensions, workmanship, and finished quality of injection molded poly vinyl chloride (PVC) profile sections used for the field fabrication of a PVC liner inside existing man-entry size circular and non-circular sewers; circular, non-circular, and box culverts, conduits, and vertical shafts or manholes having dimensions of 39.4 in. and larger (1000 mm and larger).1.2 The segmental panel system produced under this specification is for non-pressure applications where the PVC liner is installed in the existing structure and the annular space between the liner and the existing structure is grouted with a low viscosity, high strength cementitious grout.1.3 Units—The values stated in either SI units or inch-pound units are to be regarded separately as standard. The values stated in each system may not be exact equivalents; therefore, each system shall be used independently of the other. Combining values from the two systems may result in non-conformance with the standard.1.4 This standard does not purport to address all of the safety concerns, if any, associated with its use. It is the responsibility of the user of this standard to establish appropriate safety, health, and environmental practices and determine the applicability of regulatory limitations prior to use.1.5 This international standard was developed in accordance with internationally recognized principles on standardization established in the Decision on Principles for the Development of International Standards, Guides and Recommendations issued by the World Trade Organization Technical Barriers to Trade (TBT) Committee.

定价： 590元 加购物车

定价： 590元 加购物车

4.1 The degree of deacetylation of chitosan, as well at the molar mass and molar mass distribution, determines the functionality of chitosan in an application. For instance, functional and biological effects are highly dependent upon the composition and molar mass of the polymer.4.2 This test method describes procedures for measurement of molar mass of chitosan chlorides and glutamates, and chitosan base, although it in principle applies to any chitosan salt. The measured molar mass is that for chitosan acetate, since the mobile phase contains acetate as counter ion. This value can further be converted into the corresponding molar mass for the chitosan as a base, or the parent salt form (chloride or glutamate).4.3 Light scattering is one of very few methods available for the determination of absolute molar mass and structure, and it is applicable over the broadest range of molar masses of any method. Combining light scattering detection with size exclusion chromatography (SEC), which sorts molecules according to size, gives the ability to analyze polydisperse samples, as well as obtaining information on branching and molecular conformation. This means that both the number-average and mass-average values for molar mass and size may be obtained for most samples. Furthermore, one has the ability to calculate the distributions of the molar masses and sizes.4.4 Multi-angle laser light scattering (MALS) is a technique where measurements of scattered light are made simultaneously over a range of different angles. MALS detection can be used to obtain information on molecular size, since this parameter is determined by the angular variation of the scattered light. Molar mass may in principle be determined by detecting scattered light at a single low angle (LALLS). However, advantages with MALS as compared to LALLS are: (1) less noise at larger angles, (2) precision of measurements is improved by detecting at several angles, and (3) the ability to detect angular variation allows determination of size, branching, aggregation, and molecular conformation.4.5 Size exclusion chromatography uses columns, which are typically packed with polymer particles containing a network of uniform pores into which solute and solvent molecules can diffuse. While in the pores, molecules are effectively trapped and removed from the flow of the mobile phase. The average residence time in the pores depends upon the size of the solute molecules. Molecules that are larger than the average pore size of the packing are excluded and experience virtually no retention; these are eluted first, in the void volume of the column. Molecules, which may penetrate the pores will have a larger volume available for diffusion, they will be retained in the column for a time dependent upon their molecular size, with smaller molecules eluting after larger molecules.4.6 For polyelectrolytes, dialysis against the elution buffer has been suggested, in order to eliminate Donnan-type artifacts in the molar mass determination by light scattering (1, 2).5 However, in the present method, the size exclusion chromatography step preceding the light scatter detection is an efficient substitute for a dialysis step. The sample is separated on SEC columns with large excess of elution buffer for 30 to 40 min, and it is therefore in full equilibrium with the elution buffer when it reaches the MALS detector.1.1 This test method covers the determination of the molar mass of chitosan and chitosan salts intended for use in biomedical and pharmaceutical applications as well as in tissue engineered medical products (TEMPs) by size exclusion chromatography with multi-angle laser light scattering detection (SEC-MALS). A guide for the characterization of chitosan salts has been published as Guide F2103.1.2 Chitosan and chitosan salts used in TEMPs should be well characterized, including the molar mass and polydispersity (molar mass distribution) in order to ensure uniformity and correct functionality in the final product. This test method will assist end users in choosing the correct chitosan for their particular application. Chitosan may have utility as a scaffold or matrix material for TEMPs, in cell and tissue encapsulation applications, and in drug delivery formulations.1.3 The values stated in SI units are to be regarded as standard. No other units of measurement are included in this standard.1.4 This standard does not purport to address all of the safety concerns, if any, associated with its use. It is the responsibility of the user of this standard to establish appropriate safety, health, and environmental practices and determine the applicability of regulatory limitations prior to use.1.5 This international standard was developed in accordance with internationally recognized principles on standardization established in the Decision on Principles for the Development of International Standards, Guides and Recommendations issued by the World Trade Organization Technical Barriers to Trade (TBT) Committee.

定价： 590元 加购物车

定价： 646元 加购物车

4.1 In this guide, the conditions, measurement apparatus, and procedures for measuring several characteristics of nanoparticle properties on three different instrument platforms using laser-amplified detection/power spectrum analysis (LAD/PSA) technology are described. This is a more recently developed technology, commercialized in 1990, than the older technology known as either photon correlation spectroscopy (PCS) or quasi-elastic light scattering (QLS)—those titles are interchangeable—developed first in 1961. Nanoparticle tracking analysis (NTA) is the most recent DLS technology to be commercialized. All three of these technologies fall under the broader category of DLS, based on the “dynamic” movement of the measured nanoparticles under Brownian motion.4.2 DLS in the lower end of the nanometre size range becomes progressively more difficult as the particle optical scattering coefficients drop sharply, reducing the scattered light intensity. The advantage of the heterodyne detection mode over the homodyne detection mode, especially at the low end of the nanometre range, will be explained.4.3 The LAD/PSA technology will be described and the major differences between it and the PCS-QLS and NTA technologies will be made clear. For thorough discussions of PCS-QLS, refer to Guide E2490, Test Method E3247, and ISO 22412 Annex Section A.1. For a thorough discussion of nanoparticle tracking analysis (NTA), refer to Guide E2834. For detailed information on laser-amplified detection/frequency power spectrum (LAD/FPS) technology, refer to ISO 22412 Annex Section A.2. General information on particle characterization practices can be found in Practice E1817, and nanotechnology terminology is given in Terminology E2456. Detailed information on sampling for particle characterization can be found in ISO 14488.1.1 The technology, laser-amplified detection/power spectrum analysis (LAD/PSA), is available in three different platforms, which will be designated as Platforms A, B, and C.1.1.1 Platform A—This is a solid-state probe configuration that serves as the optical bench in each of the platforms. It consists of an optical fiber coupler with a y-beam splitter that directs the scattered light signal from the nanoparticles at 180° back to a photodiode detector. The sensing end of the probe can be immersed in a suspension or positioned to measure one drop of a sample on top of the sensing surface.1.1.2 Platform B—The same probe is mounted in a case, positioned horizontally, to detect the signal from either a disposable or permanent cuvette.1.1.3 Platform C—Two probes are mounted in a case, horizontally, at opposite sides of a permanent sample cell. Both size distribution and zeta potential can be measured in this configuration.1.2 The laser beam travelling through the probe measuring the scattered light from the sample of nanoparticles, in all three platforms, is partially reflected back to the same photodiode detector, and the high optical power of the laser is added to the low optical power of the scattered light signal. The interference (mixing or beating) of those two signals is known as heterodyne beating. The resulting high-power detected signal provides the highest signal-to-noise ratio among dynamic light-scattering (DLS) technologies.1.3 This combined, amplified, optical signal is converted with a Fast Fourier transform (FFT) into a frequency power spectrum, then into a logarithmic power spectrum that is deconvolved into number and volume size distributions. The mean intensity, polydispersity, number and volume size distributions, concentration, and molecular weight can be reported in all platforms, plus zeta potential on Platform C.1.4 This technology is capable of measuring nanoparticles in a size range from 2.0 nanometres (nm) to 10 micrometres (µm), at concentrations in a suspending liquid medium up to 40 % cc/mL for all parameters given in 1.3.1.5 Units—The values stated in SI units are to be regarded as the standard. No other units of measurement are included in this standard.1.6 This standard does not purport to address all of the safety concerns, if any, associated with its use. It is the responsibility of the user of this standard to establish appropriate safety, health, and environmental practices and determine the applicability of regulatory limitations prior to use.1.7 This international standard was developed in accordance with internationally recognized principles on standardization established in the Decision on Principles for the Development of International Standards, Guides and Recommendations issued by the World Trade Organization Technical Barriers to Trade (TBT) Committee.

定价： 590元 加购物车

定价： 590元 加购物车

定价： 541元 / 折扣价： 482 元 加购物车

定价： 元 加购物车